F肌动蛋白作为胞间连丝组分的结构与生理学证据

以蒜(Allium sativum L.)瓣鞘外表皮为材料,利用荧光特异探针与共焦镜检术,结合透射电镜与免疫金标记对表皮细胞间胞间联络的性质、结构进行了系统观察.结果表明,加厚壁上的通道是由狭长的管状胞质和初生纹孔场上成束的胞间连丝衔接组成,前者实为原生质体的一部分.单个胞间连丝的孔径为60～70 nm,属正常胞间连丝范围,它们乃相邻细胞间共质联系的所在.荧光探针TRITC-Phalloidin (TRITC-Ph)标记的结果显示,整个通道上呈现红色荧光的纤索在接近初生纹孔场处明显变窄,与超微结构观察中所见的结构特点相吻合,共焦镜下观察到的初生壁上的荧光亮斑乃初生纹孔场中成束胞间连丝被标记的反映,从而有效地证实了F肌动蛋白在常态胞间连丝上的存在.免疫金标记实验显示在管状胞质中和胞间连丝上有金颗粒分布,这一结果为证实荧光标记物具肌动蛋白性质提供了有说服力的补充.     

F—肌动蛋白是蒜根端分生组织细胞核和染色体的组成成分

以兔抗鸡肌动蛋白抗体为一抗、ＦＩＴＣ羊抗兔ＩｇＧ抗体为二抗进行间接免疫荧光标记实验,观察到蒜（ＡｌｉｕｍｓａｔｉｖｕｍＬ．）根端分生组织细胞核和染色体均发出明亮的黄绿色荧光,说明其中含有肌动蛋白。经ＴＲＩＴＣ鬼笔环肽标记后,完整的间期细胞、游离的间期细胞核、前期和中期染色体以及末期子细胞核均发出较强的红色荧光,而固定前用细胞松弛素Ｄ处理的根端分生组织细胞的荧光明显减弱或没有荧光,这些结果说明细胞核和染色体中存在着Ｆ肌动蛋白。抗肌动蛋白抗体和鬼笔环肽双标记实验结果指出,同一细胞核和染色体,在ＦＩＴＣ的激发光波长下发出代表总肌动蛋白的黄绿色的ＦＩＴＣ型荧光,在ＴＲＩＴＣ的激发光波长下则发出代表Ｆ肌动蛋白的红色的ＴＲＩＴＣ型荧光,两类荧光的分布是一致的。上述结果进一步证明Ｆ肌动蛋白是细胞核和染色体的组成成分,并说明Ｆ肌动蛋白可能是细胞核和染色体中肌动蛋白的主要存在方式。     

Bacillus cereus B-02对Botrytis cinerea 拮抗机理的研究

采用电子显微镜(扫描、透射)和激光扫描共聚焦显微镜,从细胞形态学和生理学水平上研究蜡样芽孢杆菌Bacillus cereus B-02过滤液对灰葡萄孢菌Botrytis cinerea的拈抗机理.结果表明,处理菌丝表面形态受到严重破坏,发牛强烈变形;荫丝细胞核、线粒体和细胞壁等哑细胞结构发生了明显改变,细胞内出现大量无膜透明内含物,并产生较人液泡.此外,处理菌丝DNA、线粒体膜电位和活性氧荧光强度均低于对照组,且差异极显著;说明B-02菌株对病原真菌菌丝细胞DNA的合成、线粒体膜电位和活性氧水平有重要影响.     

Bacillus cereus B-02对Botrytis cinerea拮抗机理的研究

采用电子显微镜(扫描、透射)和激光扫描共聚焦显微镜,从细胞形态学和生理学水平上研究蜡样芽孢杆菌Bacillus cereus B-02过滤液对灰葡萄孢菌Botrytis cinerea的拮抗机理。结果表明,处理菌丝表面形态受到严重破坏,发生强烈变形;菌丝细胞核、线粒体和细胞壁等亚细胞结构发生了明显改变,细胞内出现大量无膜透明内含物,并产生较大液泡。此外,处理菌丝DNA、线粒体膜电位和活性氧荧光强度均低于对照组,且差异极显著;说明B-02菌株对病原真菌菌丝细胞DNA的合成、线粒体膜电位和活性氧水平有重要影响。     

蒜鳞片休眠进程中胞间联络的变化及类外连丝结构与功能的研究

利用电子显微镜术,对蒜休眠进程中鳞片薄壁细胞间胞间联络的特征进行了实验观察,发现不同时期胞间联络具有随细胞间生理关系密切程度而呈现相应结构变化的特点。并观察到萌芽期鳞片中衰败细胞与存活细胞之间有类外连丝型胞间连丝的存在;以激光共聚焦荧光显微镜结合荧光标记物示踪检测,发现不透膜荧光物质分子量为457Da 的萤黄(Lucifer yellow,LYCH),可以共质体运输方式进入存活细胞内,论证了类外连丝这一胞间连丝特定修饰态的存在,并可在一段时间内继续保持生理活性,起到进行物质共质运输的功能。     

细胞内微丝骨架的变化对人肝癌Bel-7402细胞形态的影响

癌细胞的形态及癌细胞的生物学行为(如粘附、迁移和浸润)与细胞内骨架系统密切相关,本研究利用Phalloidin-FTTC标记人肝癌Bel-7402细胞内F-肌动蛋白(F-aetin),使用激光扫描共聚焦显微镜观测细胞微丝骨架与癌细胞形态的关系,及Cyt-B处理Bel-7402细胞后,癌细胞内微丝骨架的变化。结果显示：癌细胞内F-aedn解聚,F-aetin小体的聚集重组是癌细胞的形态变化的主要因素之一。     

组织中肥大细胞内F—actin对其不同亚型细胞分泌作用的影响

目的:研究细胞内丝状肌动蛋白的变化对不同亚型肥大细胞分泌作用的影响.方法: 利用肥大细胞的特征性蛋白酶抗体和鬼比环肽的免疫荧光标记;以流式细胞仪检测分选人皮肤组织中肥大细胞的亚型;使用激光扫描共聚焦显微镜显示肥大细胞内分泌颗粒和微丝的分布.结果:类胰蛋白酶免疫反应性的肥大细胞内含有丰富的丝状肌动蛋白环,在质膜内层区域形成阻碍类胰蛋白酶释放的屏障;大量的类胰蛋白酶暂存于分泌泡中,少量的类胰蛋白酶因细胞内丝状肌动蛋白环的解聚使之从分泌泡中释放.而类胰蛋白酶和类糜蛋白酶免疫反应性的肥大细胞及类糜蛋白酶免疫反应性的肥大细胞内少见或未见明显的阻碍蛋白酶释放的丝状肌动蛋白环;细胞形态膨胀,细胞内蛋白酶已释放.结论:人皮肤组织中肥大细胞内类胰蛋白酶和/或类糜蛋白酶的含量及其肥大细胞亚型与丝状肌动蛋白环相关联.     

肌动蛋白相关蛋白2/3复合体的结构、功能与调节

微丝参与了细胞形态维持及细胞运动等多种重要的细胞过程。微丝由肌动蛋白单体组装而成 ,肌动蛋白相关蛋白 2 / 3(Arp2 /Arp3,Arp2 / 3)复合体在微丝形成过程中起重要作用。Arp2 / 3复合体由 7个亚单位组成 ,在细胞内受到多种核化促进因子的调节 ,并与这些因子协同作用来调节肌动蛋白的核化。Arp2 / 3复合体结构、功能及调节的研究对于阐明微丝形成机制及细胞骨架与某些信号分子的关系有重要意义。     

核仁骨架(核仁基质)的结构与成分——肌动蛋白与fibrillarin是核仁骨架的主要成分

将分离纯化的HeLa细胞核仁经非离子去垢剂、核酸酶、低盐及高盐选择性抽提结合DGD包埋去包埋技术 ,在电镜下显示了HeLa细胞的核仁骨架呈精细网络结构 .BHK -2 1细胞及小鼠肝细胞的核仁骨架与HeLa细胞的核仁骨架结构相类似 .对HeLa细胞的核仁骨架的蛋白成分进行了分析 .结果表明核仁骨架蛋白组成与核基质及染色体骨架有明显差异 .HeLa细胞核仁骨架的蛋白成分主要包括分子量为48,43,36及 33ku左右的 6～ 7种多肽 .证明分子量为 43ku的肌动蛋白与 36ku的fibrillarin是构成核仁骨架的两种主要蛋白成分     

Confocal Fluorescence Microscopic Observation on the Transcellular Distribution of Actin Filaments in the Epidermis of Garlic Clove Sheath

By means of paraformaldehyde fixation, Triton X-100 extraction and TRITC-phalloidin staining, the presence and distribution patterns of F-actin in the outer epidermal cells of the garlic (Allium sativum L.) sheath were studied with fluorescence probe technique and confocal laser scanning microscopy. There were a lot of actin filaments (AFs) impenetrate the cell wall, but the AFs with red fluorescence were absent when the cells were treated with cytochalasin D before fixation; the same result was obtained when the cells were treated with unlabeled phalloidin. These results indicate the presence of F-actin in the intercellular channels and that it is related to the plasmodesmata and intercellular trafficking of macromolecules.     

共聚焦荧光镜检术揭示大蒜鳞片细胞间期核中的F肌动蛋白网络

采用免疫荧光和荧光分子探针技术与共聚焦激光扫描显微镜观察相结合,对大蒜（Ａｌｌｉｕｍ ｓａｔｉｖｕｍ Ｌ．）鳞片细胞间期核中是否存在Ｆ肌动蛋白进行了研究。结果表明,以兔抗肌动蛋折抗体为一抗、ＦＴＴＧ－羊抗兔ＩｇＧ抗体为二抗进行免疫荧光标记实验,在荧光镜下观察到蒜瓣薄壁组织的细胞核及表皮细胞核均发出明亮的黄绿色荧光经共聚焦激光扫描显微镜进一步检查,整个细胞核呈黄绿色荧光,说明其中含有肌动蛋白。经ＴＲ     

利用激光共聚焦扫描显微镜对溃疡病菌侵染柑橘叶片的实时观察

柑橘溃疡病对柑橘产业造成了巨大损失,而研究柑橘与溃疡病菌的互作关系以及柑橘的感病和抗病性均需要观察溃疡病菌在柑橘寄主中的侵染和定殖过程。激光共聚焦扫描显微镜不仅可以观察活细胞,活组织的动态代谢过程,而且可以获得三维图像,对于病原菌在柑橘植物组织内的繁殖和致病机制研究具有重要意义。但是,选择适宜的植物材料和制片方法对激光共聚焦扫描显微镜的观察效果影响很大。本文对激光共聚焦扫描显微镜所观察的材料在其处理和观察方法上加以改进,获得了质量更好的图片和实验结果,也使得实验更为方便快捷。激光共聚焦扫描显微观察还在瞬时表达分析中得到应用,提高了柑橘瞬时表达分析的效果。通过将切片和压片相结合观察到溃疡病菌在不同时间点对柑橘叶片的侵染情况,而通过3D建模能观察到柑橘叶片不同组织层面中的病菌数量和病菌位置,为研究溃疡病菌在叶片中的定殖方式和入侵数量提供了前期基础。     

Visualization of alginate-poly-L-lysine-alginate microcapsules by confocal laser scanning microscopy

Confocal laser scanning microscopy (CLSM) was used to study the distribution of polymers and cross-linking ions in alginate-poly-L-lysine (PLL) -alginate microcapsules made by fluorescent-labeled polymers. CLSM studies of Ca-alginate gel beads made in the presence and absence of non-gelling sodium ions revealed a more inhomogeneous distribution of alginate in beads formed in the absence of non-gelling ions. In the formation of alginate-PLL capsules, the polymer gradients in the preformed gel core were destabilized by the presence of non-gelling ions in the washing step and in the PLL solution. Ca-alginate gels preserved the inhomogeneous structure by exposure to ion-free solution in contrast to exposure to non-gelling ions (Na(+)). By exchanging Ca(2+) with Ba(2+) (10 mM), extremely inhomogeneous gel beads were formed that preserved their structure during the washing and exposure to PLL in saline. PLL was shown to bind at the very surface of the alginate core, forming a shell-like membrane. The thickness of the PLL-layer increased about 100% after 2 weeks of storage, but no further increase was seen after 2 years of storage. The coating alginate was shown to overlap the PLL layer. No difference in binding could be observed among coating alginates of different composition. This paper shows an easy and novel method to study the distribution of alginate and PLL in intact microcapsules. As the labeling procedures are easy to perform, the method can also be used for a variety of other polymers in other microencapsulation systems.     

Flow cytometry and live confocal analysis for the evaluation of the uptake and intracellular distribution of FITC-ODN into HaCaT cells

In this study, the mechanism of the internalization and the cellular distribution of 59 fluorescein conjugated PS-ODN (FITC-ODN) after transfection with different mixed lipidic vesicles/oligo complexes (lipoplexes) have been investigated. Mixed lipidic vesicles were prepared with one of the most used cationic lipid (DOTAP) and different amounts of a cholic acid (UDCA) to release the oligo into HaCaT cells. Using flow cytometry, the cellular uptake of the oligo was studied with and without different inhibitors able to block selectively the different pathways involved in the internalization mechanism. The intracellular distribution of the oligo was analyzed by confocal laser scanning microscopy (CLSM), treating the cells with the lipoplexes and directly observing without any fixing procedure. To better carry out the colocalization studies, fluorescent-labeled markers, specific for the different cellular compartments, were coincubated with 59 fluorescein-conjugated 29-mer phosphorotioate oligonucleotide (FITC-ODN). The different lipidic vesicles affect the internalization mechanism of FITC-ODN. After using the inhibitors, the uptake of complexes involved a different internalization mechanism. The live CLSM analysis demonstrated that, after 1 hour from the complex incubation, the oligo was transferred into cells and localized into the endosomes; after 24 hours, the oligo was intracellularly localized close to the nuclear structure in a punctuate pattern. However, the results from fusion experiments showed also a binding of a quite low amount of oligo with the cell membranes.     

巴西固氮螺菌Yu62在玉米根的定植

将GFPmut2质粒中的gfp基因(编码绿色荧光蛋白)克隆到载体pVK100中,构建成重组质粒pVK1001。将pVK1001通过电转化方法导入到联合固氮菌巴西固氮螺菌Yu62中,获得GFP)标记的巴西固氮螺菌Yu62菌株。用标记菌株接种限菌培养条件下生长的玉米(农大3318)幼苗,在接种后8d、12d,用激光共聚焦扫描显微镜进行观测,结果表明巴西固氮螺菌Yu62菌株能定植于玉米根部皮层的薄壁细胞间隙。用扫描电镜和超薄切片电镜观察表明,大多数细菌主要定植于根表,少数菌可进入玉米根组织内。     

Revealing the F_actin Networks in Interphase Nuclei of Garlic Clove Cells by Confocal Fluorescence Microscopy

The interphase nuclei of parenchyma cells and epidermal cells of garlic (Allium sativum L.) clove were labelled with rabbit anti-actin antibody and FITC-conjugated goat anti-rabbit IgG antibody. The authors observed results with fluorescence microscopy and confocal laser scanning microscopy. The nuclei showed prominent green-yellow fluorescence, indicating the presence of actin in the nuclei. Fluorescence examination with TRITC-phalloidin showed distinctive red fluorescence in the nuclei, indicating that F-actin is present in the nuclei. Confocal laser scanning microscopy indicated the presence of F-actin containing network structures in the nuclei, but the network structures were absent and the nuclei still showed red fluorescence when the cells were treated with cytochalasin D before fixation; the red fluorescence in the nuclei was hard to be observed when the cells were treated with unlabelled phalloidin before the cells were stained with TRITC-phalloidin. These results indicate that F-actin is in the nuclei and forms network structures in the nuclei of garlic cells.     

巴西固氮螺菌Yu62在玉米根的定植

将GFPmut2质粒中的gfp基因 (编码绿色荧光蛋白)克隆到载体pVK100中,构建成重组质粒pVK1001.将pVK1001通过电转化方法导入到联合固氮菌巴西固氮螺菌Yu62中,获得GFP标记的巴西固氮螺菌Yu62菌株.用标记菌株接种限菌培养条件下生长的玉米(农大3318)幼苗,在接种后8 d、12 d,用激光共聚焦扫描显微镜进行观测,结果表明巴西固氮螺菌Yu62菌株能定植于玉米根部皮层的薄壁细胞间隙.用扫描电镜和超薄切片电镜观察表明,大多数细菌主要定植于根表,少数菌可进入玉米根组织内.