光增白剂M2R对草地螟中肠围食膜的影响及对Bt毒力的增效作用

以光增白剂M2R作为影响因子,探讨其对草地螟Loxostege sticticalis幼虫围食膜（peritrophic membrane, PM）的作用机理。通过环境扫描电镜观察和生化测定研究了光增白剂对草地螟幼虫围食膜结构和蛋白质种类的影响,及其对Bt毒力的增效作用。结果表明：围食膜含有多种蛋白质,经SDS-PAGE测定至少有19条带,分子量在94 kD以下,虫取食光增白剂可影响围食膜中几丁质结合蛋白（chitin binding proteins,CBPs）的含量。不同浓度的光增白剂可以对草地螟围食膜的形态结构产生明显的影响,正常的围食膜表面光滑致密、无孔洞和缝隙,增白剂处理的围食膜产生了孔缝。生测实验表明,添加光增白剂后能够显著缩短Bt的杀虫时间 降低Bt的使用浓度。可见,光增白剂可对草地螟围食膜产生损伤,进而提高了Bt的防治效果。     

天然产物梣酮对粘虫围食膜的影响

【目的】梣酮是从芸香科植物白鲜Diatamnus dasycarpus根皮中分离出的一种化合物, 对试虫表现出胃毒活性。本研究旨在检测梣酮对粘虫Mythimna separata 6龄幼虫中肠围食膜的影响, 从而进一步阐明梣酮的杀虫作用机理。【方法】经活体及离体处理, 通过生化分析和扫描电镜观察等方法, 研究了梣酮处理对粘虫幼虫中肠围食膜糖含量, 蛋白质含量和组分以及围食膜表面结构的影响。【结果】梣酮(20 mg/mL)活体处理降低了粘虫6龄幼虫围食膜的蛋白质含量, 却使糖含量升高。活体(20 mg/mL梣酮)及离体(8 mg/mL梣酮)处理条件下, 围食膜糖含量分别为对照组的1.75倍及2.17倍。SDS-PAGE结果显示, 离体及活体条件下经梣酮处理, 围食膜部分蛋白质降解。围食膜解剖扫描电镜观察表明, 梣酮处理可造成围食膜微纤丝排列紊乱。【结论】天然产物梣酮处理对粘虫中肠围食膜的糖含量及蛋白质含量和组分有影响,且改变了围食膜表面结构。本研究为深入地研究梣酮杀虫作用机理奠定了基础。     

围食膜: 害虫生物防治的潜在靶标

围食膜是昆虫中肠细胞分泌的一层特有的非细胞结构,由蛋白质、粘多糖和几丁质组成,是昆虫中肠细胞抵御随食物摄入的病原微生物入侵的第一道天然屏障。昆虫病毒增效蛋白、几丁质酶、荧光增白剂和外源凝集素等生物防治促进因子通过与围食膜上特异位点的结合,可破坏围食膜结构,改变其通透性,促进病原微生物对害虫的感染。该文综述了与昆虫围食膜密切相关的生防促进因子的增效活性及其作用机理,阐明了以围食膜为害虫生物防治靶标的应用前景。     

昆虫体内的天然屏障——围食膜

昆虫围食膜是由昆虫中肠上皮细胞分泌的非细胞薄膜状结构,主要成份是几丁质、蛋白质和多糖,是昆虫抵御外界侵害的第一道天然屏障,能够保护中肠上皮细胞不受机械损伤并且能够抵御病毒、细菌及其他有害物质,防止化学损伤.昆虫病毒增效蛋白、荧光增白剂和几丁质酶等生物防治促进因子通过与围食膜上特异位点的结合,能够破坏围食膜结构,加速病原微生物对害虫的感染进程.就围食膜组分、结构、功能以及与害虫防治的关系等方面的研究进展进行综述,并且论述了以围食膜为害虫生物防治靶标的应用前景.     

昆虫中肠围食膜蛋白研究进展

围食膜是大多数昆虫中肠内壁附着的一层起润滑和保护作用的半透性粘膜, 按其形成方式不同分为Ⅰ型围食膜和Ⅱ型围食膜。围食膜主要由几丁质和蛋白质构成, 其中蛋白质对于维持围食膜的致密结构至关重要, 对围食膜蛋白的破坏可能会对昆虫的正常生长发育造成干扰, 甚至会导致低龄幼虫的死亡。本文介绍了围食膜的组成与结构, 阐述了昆虫围食膜蛋白研究的新发现、并依据结构特征对它们进行了分类, 总结了以围食膜蛋白为新靶标的害虫防治的可能途径, 讨论了当前围食膜蛋白研究的不足, 最后展望了今后围食膜蛋白研究的发展方向。     

棉铃虫围食膜蛋白的电泳分离技术

比较了棉铃虫Helicoverpa armigera(Hübner)围食膜不同处理方法,不同围食膜数量,在不同电泳下的分离效果,筛选最佳的围食膜蛋白分离技术。结果表明:冷冻干燥与非冷冻干燥处理围食膜后进行SDS-PAGE电泳分离效果基本相同,建议使用冷冻干燥后处理较好。取1、3、5条围食膜进行SDS-PAGE电泳,都能将围食膜蛋白分离,且分离效果基本一致,建议5条围食膜最合适,具有可靠性和代表性。浓缩胶为5%、分离胶分别为8%、10%和12%时棉铃虫围食膜的SDS-PAGE电泳分离效果差异不大,而分离胶为12%时效果较好。无水三氟利克酸处理围食膜后进行NuPAGE电泳,分离出的围食膜蛋白大约30多种,远远超过上述方法分离的16²0种,且需要的围食膜材料少,分离效果最佳,但费用高。     

棉铃虫围食膜的蛋白质组鉴定

【目的】围食膜(peritrophic membrane, PM)是昆虫抵御随食物摄入的病原微生物入侵的第一道天然屏障。本研究旨在鉴定出农业重大害虫棉铃虫Helicoverpa armigera围食膜的总蛋白成分,为进一步揭示昆虫围食膜的形成机制及研发新颖的害虫控制策略奠定基础。【方法】剥离棉铃虫5龄幼虫PM,用三氟甲磺酸(trifluoromethane sulfonic acid, TFMS)处理,采用液质联用技术(LC-MS/MS)鉴定围食膜蛋白质组,然后对鉴定结果进行生物信息学分析。【结果】本研究共鉴定出棉铃虫幼虫围食膜蛋白质169个,是目前鉴定最多的棉铃虫围食膜蛋白。通过GO分析,可以将这些鉴定的蛋白分为细胞组分、分子功能和生物学过程三大类;KEGG富集结果显示,鉴定蛋白可以富集在12条代谢通路中;蛋白互作分析(protein protein interaction, PPI)结果表明,以ACC和CG3011等蛋白为核心可以形成蛋白互作网络。【结论】本研究鉴定了169个棉铃虫幼虫围食膜蛋白质,并对其进行了GO, KEGG和PPI分析,结果有助于人们全面理解昆虫围食膜的分子结构和功能。     

刚果红对棉铃虫中肠围食膜的影响及其病毒增效作用

通过观察棉铃虫幼虫正常围食膜（peritrophic membrane, PM）的形态、结构和组成,研究了刚果红对棉铃虫幼虫围食膜的破坏作用及其对棉铃虫核多角体病毒（HaNPV）的增效作用。结果表明,棉铃虫的围食膜分布于整个中肠,包裹着食物呈液囊状,类似于Ⅰ型围食膜;健康的围食膜呈无色、透明网状结构,并具有一定韧性,经刚果红染色后呈现桔红色。使用不同浓度梯度的刚果红喂食5龄幼虫,结果显示摄取含1.5%和2.0%刚果红的饲料2.5 h后,宿主不能形成完整的围食膜,而是形成易脆无弹性的围食膜碎片。经过恢复实验后发现,刚果红对围食膜的破坏作用是瞬时的,可以在较短时间内得到修复。用1.0%刚果红喂食初孵幼虫,发现1.0%刚果红对棉铃虫的幼虫生长不能产生明显的影响。1.0％刚果红能加强棉铃虫幼虫对HaNPV的敏感性,缩短病毒杀虫时间,能使5龄幼虫的病毒感染致死率达到63％,对HaNPV具有非常显著的增效作用。     

昆虫围食膜的研究进展

围食膜是大多数昆虫中肠内的半透性薄膜 ,主要由几丁质、蛋白质构成。依据其形成的方式分 :Ⅰ型围食膜 ,由整个中肠细胞分泌形成多层管状膜 ;Ⅱ型围食膜由中肠前端特殊的细胞分泌成连续的套筒管状膜。由于位于食物与中肠上皮细胞间而在中肠生理中起重要作用 ,围食膜保护中肠上皮免于机械损伤以及病原菌、毒素的入侵 ;作为半透膜以及将中肠分为不同的区室而在营养物质的消化和吸收中具有重要作用。该文综述了有关围食膜结构、组分、功能、通透性以及与害虫防治的关系等方面的研究进展。     

有色膜遮光对烤烟生长和光合特性及其初烤品质的影响

以自然光为对照,采用红色、白色、蓝色、黄色4种有色薄膜于2010~2011年从团棵期开始对大田烤烟进行遮光处理,研究不同光质对烤烟生长、光合特性及初烤品质指标的影响。结果显示:(1)红膜处理最大叶长宽比最小、叶面积最大,黄膜处理则相反。(2)红、蓝膜处理烟叶净光合速率、气孔导度、蒸腾速率明显高于自然光处理,白、黄膜处理略高于对照或与对照持平,且遮膜处理前期红膜高于蓝膜处理,后期蓝膜高于红膜处理。(3)红、蓝膜处理有利于提高倒5叶SPAD值,黄膜处理则相反。(4)红膜处理显著降低了中部叶蛋白质、总氮含量和氮碱比,提高了施木克值,并显著提高了上部叶可溶性糖含量和氮碱比,降低了施木克值;蓝膜处理显著提高了中部叶烟碱和多酚含量,降低了可溶性糖含量、施木克值及氮碱比,并显著提高了上部叶蛋白质、总氮、烟碱和多酚含量,降低了施木克值,提高了氮碱比;黄膜处理显著降低了中上部叶蛋白质、总氮、烟碱和多酚含量,提高了上部叶施木克值、降低了氮碱比。研究表明,红、蓝膜处理更利于烟叶发育和光合特性的提高,初烤烟叶化学成分更协调,利于优质烟叶的形成。     

The Morphology and Permeability of Isolated Cuticular Membranes of Hoya carnosa R. Br. (Asclepiadaceae)

This investigation is in part an extension of previous leafcuticle observations made on 52 other taxa among 34 families.Dewaxed, chemically isolated, adaxial and abaxial cuticularmembranes and transverse leaf sections of the wax-flower plant(Hoya carnosa R. Br.) were examined using ordinary stainingtechniques and light-microscopy methods. Evidence is presentedfor the existence of ubiquitous, discrete, naturally occurringcuticular pores, concomitant with anticlinally oriented trans-cuticularcanals, distributed randomly throughout the cuticular matrix.The surface of the adaxial cuticular membrane contains approx.6540 unclustered pores per mm², the abaxial approx. 4680 poresper mm². Pore and canal diameters range between 0.5 and 0.75µm. The canals are often arcuate and their lengths aredirectly related to cuticle thickness. No correlations werefound between cuticle thickness and either pore numbers or poreand canal diameters. Based upon experiments with various pHindicators, solutions, and stains, the dewaxed, dry cuticularmembrane of H. carnosa appears to be both distinctly hydrophilicand selectively permeable through a myriad of microscopicallyvisible pores and canals permeating its matrix. A de novo interpretationof gross cuticle morphology based solely upon light microscopyobservations is presented by semi-diagrammatic illustrations. Hoya carnosa R. Br., wax-flower (wax-plant), cuticular membranes, cuticular pores, transcuticular canals, permeability     

Forskolin-induced apical membrane insertion of virally expressed, epitope-tagged CFTR in polarized MDCK cells

Channel gating ofthe cystic fibrosis transmembrane conductance regulator (CFTR) isactivated in response to cAMP stimulation. In addition, CFTR activationmay also involve rapid insertion of a subapical pool of CFTR into theplasma membrane (PM). However, this issue has been controversial, inpart because of the difficulty in distinguishing cell surface vs.intracellular CFTR. Recently, a fully functional, epitope-tagged formof CFTR (M2-901/CFTR) that can be detected immunologically innonpermeabilized cells was characterized (Howard M, Duvall MD,Devor DC, Dong J-Y, Henze K, and Frizzell RA. Am J PhysiolCell Physiol 269: C1565-C1576, 1995; and Schultz BD,Takahashi A, Liu C, Frizzell RA, and Howard M. Am J PhysiolCell Physiol 273: C2080-C2089, 1997). We have developedreplication-defective recombinant adenoviruses that expressM2-901/CFTR and used them to probe cell surface CFTR in forskolin(FSK)-stimulated polarized Madin-Darby canine kidney (MDCK) cells.Virally expressed M2-901/CFTR was functional and was readilydetected on the apical surface of FSK-stimulated polarized MDCK cells.Interestingly, at low multiplicity of infection, we observedFSK-stimulated insertion of M2901/CFTR into the apical PM, whereas athigher M2-901/CFTR expression levels, no increase in surfaceexpression was detected using indirect immunofluorescence. Immunoelectron microscopy of unstimulated and FSK-stimulated cells confirmed the M2-901/CFTR redistribution to the PM upon FSKstimulation and demonstrates that the apically insertedM2-901/CFTR originates from a population of subapical vesicles.Our observations may reconcile previous conflicting reports regardingthe effect of cAMP stimulation on CFTR trafficking.

     

Modification of the root plasma membrane lipid composition of cadmium-treated Pisum sativum

The effects of in vivo Cd treatments on pea root plasma membrane(PM) lipid composition were studied. In the long-term experiment,plants were supplied with Cd: moderate stress (10 µM)or strong stress (50 µM) for 10 d. Growth of root andshoot was severely affected in 50 µM Cd-treated plants,as evidenced by the approximately 7-fold reduction in theirRelative Growth Increment (RGI). Treatment with Cd (10 µM)resulted in changes to the lipid composition of the pea rootPM, including increases in the degree of unsaturation of phospholipid-associatedfatty acids and in the relative amount of stigmasterol (30–42%).This change was accompanied by a reduction in sitosterol content(26.8 to 17.4 µg mg^–1 protein). However, the sterolcomposition was not altered in plants treated with 50 µMCd for 10 d. The content of phosphatidylethanolamine and phosphatidylcholine(major phospholipids present in pea root PM) decreased as Cdlevel increased, but the ratio between them remained unaffected.In the short-term experiment, plants exposed to Cd (50 µM)accumulated less sitosterol (from 27.7 to 14.0 µg g mg^–1protein) over 72 h, but no significant effect on other measuredlipids was observed. The physiological repercussions of changesin plasma membrane lipid composition, as a result of Cd exposureare discussed. Key words: Cadmium, lipids, pea, Pisum sativum, plasma membranes     

The Rate of Water-loss from Stripped Leaves

Stripping off the epidermis of Sedum leaves is found to increasethe rate of water-loss by amounts of the order of 700 per cent.A high resistance of the pores of the stomatal epidermis tothe diffusion of water-vapour from the mesophyll is thus indicated. Stripping one surface of a leaf considerably increases the rateof transpiration from the other (untouched) surface. The explanationof this is under investigation. In conclusion, the writer wishes to thank Dr. F. M. Haines forsuggestions, interest and criticism. Thanks are also due tothe staff of the Chelsea Physic Garden and to Mr. I. R. McGregorfor his valuable technical assistance.     

华北大黑鳃金龟两种围食膜蛋白cDNA的分子克隆与序列分析

本文以华北大黑鳃金龟Holotrichia oblita中肠为材料,依据Stratagene公司文库构建试剂盒方法,构建其中肠cDNA表达文库,该文库滴度为1.9×106 pfu/mL,重组率为99.97%。依据现代免疫学原理,利用棉铃虫Helicoverpa armigera围食膜蛋白多克隆抗体筛选文库,得到两个编码华北大黑鳃金龟围食膜蛋白的cDNA克隆Ho-Peritrophin1与Ho-Peritrophin2,其cDNA长分别为2 385 bp和1 633 bp,在PolyA末端上游各有3个多聚腺苷酸信号序列AATAAA,最长开放阅读框(ORF)分别编码729个和477个氨基酸,与粉纹夜蛾Trichoplusia ni CBP2(chitin binding protein 2)的相似性最高,分别为21.9%和19.1%。结构域分析表明,Ho-Peritrophin1与Ho-Peritrophin2分别具有9个和6个几丁质结合功能域,只含有较少的O-糖基化位点,不含有类粘蛋白结构域。胰蛋白酶和胰凝乳蛋白酶对两种蛋白的作用位点主要位于几丁质结合功能域(chitin binding domain, CBD)内部,而因受几丁质结合功能域保护,这两种蛋白能够抵抗这些蛋白酶的降解。与正常CBD比较,这两种蛋白C端的CBD只含有4个Cys,只在第1与第3、第4与第5个Cys之间形成两对二硫键,缺少由第2与第6个Cys形成的二硫键。推测其N端还应包括信号肽序列和几丁质结合功能域的未知序列。     

基于线粒体COI基因序列的文蛤属(软体动物门:帘蛤科)系统发育关系(英文)

测定了4种文蛤属贝类的15个个体的COI基因序列,并从GenBank下载了短文蛤 (M. petechialis)的相应序列。比对后的序列长度为574 bp,包括93个简约信息位点,A、T、C和G的平均含量分别为21.15%、44.71%、14.05%和20.09%。通过对序列的分析,共定义了12个单倍型：文蛤 (M. meretrix) 4个,斧文蛤 (M. lamarckii) 2个,丽文蛤 (M. lusoria) 3个,琴文蛤 (M. lyrata) 1个,短文蛤2个。以青蛤(Cylina sinensis)为外群,用MP法和贝叶斯法构建系统树。结果显示,短文蛤、丽文蛤和文蛤为亲缘关系较近的物种, 支持短文蛤和丽文蛤为文蛤的同物异名的观点。     

Hormonal and metabolic responses to exercise across time of day and menstrual cycle phase

Galliven, E. A., A. Singh, D. Michelson, S. Bina, P. W. Gold, and P. A. Deuster. Hormonal and metabolic responses to exercise across time of day and menstrual cycle phase.J. Appl. Physiol. 83(6):1822-1831, 1997.Two studies, each utilizing short-term treadmillexercise of a different intensity, assessed the metabolic and hormonalresponses of women to exercise in the morning (AM) and late afternoon(PM). In study 1, plasmaconcentrations of growth hormone, arginine vasopressin, catecholamines,adrenocorticotropic hormone, cortisol, lactate, and glucose weremeasured before, during, and after high-intensity exercise (90%maximal O₂ uptake) in the AM andPM. In study 2, plasma concentrationsof adrenocorticotropic hormone, cortisol, lactate, andglucose were measured before, during, and aftermoderate-intensity exercise (70% maximalO₂ uptake) in the AM and PM in thefollicular (days 3-9), midcycle (days 10-16), and luteal(days 18-26) phases of themenstrual cycle. The results of studies1 and 2 revealed nosignificant diurnal differences in the magnitude of responses for anymeasured variable. In addition, study2 revealed a significant time-by-phase interaction forglucose (P = 0.014). However, netintegrated responses were similar across cycle phases. These datasuggest that metabolic and hormonal responses to short-term,high-intensity exercise can be assessed with equal reliability in theAM and PM and that there are subtle differences in blood glucoseresponses to moderate-intensity exercise across menstrual cycle phase.

     

Somatic Hybrids of the Forage Legumes Medicago sativa L. and M. falcata L.

Protoplasts isolated from embryogenic cell suspensions of tetraploidMedicago sativa cv. Europe (2n= 4? = 32) and M. falcata (2n=4? = 32) were fused using polyethylene glycol (PEG). Heterokaryonswere isolated by micromanipulation and cultured in the presenceof nurse protoplasts from albino or embryogenic cell suspensionsof M. sativa, to give free-floating embryos and embryogeniccalli. Ninety-nine plants were regenerated from somatic embryos.Fifteen of the plants exhibited leaf abnormalities and did notsurvive transfer from culture to the glasshouse. The remainingphenotypically normal plants were established ex vitro and floweredat maturity. Morphological and biochemical analyses confirmedthat 12 of the phenotypically normal plants were somatic hybrids.Morphological characteristics of the hybrids, including plantstature, internode length, leaf size, flower colour, and podshape, were intermediate compared with those of the purple floweredM. sativa and yellow flowered M. falcata parents. Flowers ofthe hybrids were yellow traced with purple-blue veins. Isoenzymebanding patterns for esterase showed bands additional to thoseof M. sativa and M. falcata. The chromosome complements of individualhybrids varied from (2n= 4? = 32) to 58.     

Water transport and the distribution of aquaporin-1 in pulmonary air spaces

Effros, R. M., C. Darin, E. R. Jacobs, R. A. Rogers, G. Krenz, and E. E. Schneeberger. Water transport and thedistribution of aquaporin-1 in pulmonary air spaces.J. Appl. Physiol. 83(3): 1002-1016, 1997.Recent evidence suggests that water transport between the pulmonary vasculature and air spaces can be inhibited byHgCl₂, an agent that inhibitswater channels (aquaporin-1 and -5) of cell membranes. In the presentstudy of isolated rat lungs, clearances of labeled(³HOH) and unlabeled water werecompared after instillation of hypotonic or hypertonic solutions intothe air spaces or injection of a hypotonic bolus into the pulmonaryartery. The clearance of ³HOHbetween the air spaces and perfusate after intratracheal instillation and from the vasculature to the tissues after pulmonary arterial injections was invariably greater than that of unlabeled water, indicating that osmotically driven transport of water is limited bypermeability of the tissue barriers rather than the rate of perfusion.Exposure to 0.5 mM HgCl₂ in theperfusate and air-space solution reduced the product of the filtrationcoefficient and surface area(P_fS)of water from the air spaces to the perfusate by 28% afterinstillation of water into the trachea. In contrast, perfusion of 0.5 mM HgCl₂ in air-filled lungs reducedP_fSof the endothelium by 86% after injections into the pulmonary artery, suggesting that much of the action of this inhibitor is on the endothelial surfaces. Confocal laser scanning microscopy demonstrated that aquaporin-1 is on mouse pulmonary endothelium. No aquaporin-1 wasfound on alveolar type I cells with immunogold transmission electronmicroscopy, but small amounts were present on some type II cells.