比较三种防冰晶法对切片保存效果的影响

目的 比较冰冻切片技术中几种防冰晶方法对切片保存效果的影响。方法 分别使用液氮骤冷组织、高渗透压脱水法、单纯OCT胶包埋等几种方法后行冰冻切片、HE染色后,分别于当天、1、3、6个月后比较其染色效果,选出最佳保存方法。结果 单纯OCT包埋法在1个月后染色明显变浅,冰晶数量最多,而在3、6个月后染色基本接近背底色,冰晶面积已占据近半个视野,组织结构破坏极其严重;高渗透压脱水法在1个月后染色深度及冰晶数量上无明显变化,但3、6个月后则明显变浅,冰晶数量明显增加;而低温骤冷法在染色后的几个月,染色深度及冰晶的数量均无明显的变化,结构基本维持染色当天的状态。结论 低温骤冷法是这三种防冰晶法中最利于保存切片的方法。     

激光扫描共聚焦显微镜在医学研究中的应用

激光扫描共聚焦显微镜（Confocal laser scanning microscope,CLSM）具有高分辨率、高灵敏度、三维重建、动态分析等优点,使图像更为精确清晰和数字化。该仪器现已广泛应用于细胞生物学、生理学、病理学、遗传学和药理学等研究领域中。本文简述了激光扫描共聚焦显微镜的结构、工作原理并归纳了其在医学各领域研究中的应用。     

Embedding Thin Plant Specimens for Oriented Sectioning

Small plant structures such as small primary roots, filamentous mosses and algae are difficult to orient for sectioning since they become wavy and curl during embedding. A method is described for embedding and orienting tiny plant specimens in a glycol methacrylate resin using self-constructed flat molds. Prior to sectioning, small samples can be oriented in both the longitudinal and the transverse plane. As several samples can be sectioned simultaneously, time-consuming trimming of the blocks is reduced substantially. The efficiency of this technique has been demonstrated using the tiny roots of the model plant Arabidopsis thaliana (L.) Heynh.     

Structure brings clarity: Structured illumination microscopy in cell biology

Biological samples are three dimensional and, therefore, optical sectioning is mandatory for microscopic images to precisely show the localization or function of structures within biological samples. Today, researchers can choose from a variety of methods to obtain optical sections. This article focuses on structured illumination microscopy, which is a group of techniques utilizing a combination of optics and mathematics to obtain optical sections: A structure is imaged onto the sample by optical means and the additional information thereby encoded in the image is used to calculate an optical section from several acquired images. Different methods of structured illumination microscopy (mainly grid projection and aperture correlation) are discussed from a practical point of view, concentrating on advantages, limitations and future prospects of these techniques and their use in cell biology. Structured illumination can also be used to obtain super-resolution information if structures of higher frequency are projected onto the sample. This promising approach to super-resolution microscopy is also briefly discussed from a user's perspective.     

不同盐度下互花米草根结构的比较研究

以不同盐度下生长的互花米草(Spartina alterniflora)为材料,采用常规石蜡切片法对其根的横切结构进行显微观察,比较不同盐度下互花米草根结构的特点及变化规律,研究互花米草根对盐浸环境的适应性。观察结果显示:(1)互花米草根只有初生结构;(2)成熟根的表皮细胞基本毁坏、脱落;(3)互花米草根具有发达的外皮层和皮层通气组织,内皮层细胞壁五面加厚明显,且随盐度的升高呈先增大后减小的趋势;(4)维管柱中央被机械组织所填充,中柱鞘细胞壁也出现加厚现象。互花米草根的结构体现了其对盐浸环境的适应性特征。     

The last few milliseconds in the life of a secretory granule

We have monitored single vesicles (granules) in bovine adrenal chromaffin cells using an optical sectioning technique, total internal reflection fluorescence microscopy (TIRFM). With TIR, fluorescence excitation is limited to an optical slice near a glass/water interface. In cells located at the interface, granules loaded with fluorescent dye can be visualized near to or docked at the plasma membrane. Here we give evidence that (1) TIRFM resolves single vesicles and (2) the fluorescence signal originates from vesicles of roughly 350 nm diameter, presumably large dense core vesicles (LDCVs). (3) Diffusional spread of released vesicle contents can be resolved and serves as a convenient criterion for a fusion event. (4) We give details on vesicle properties in resting cells, such as lateral mobility of chromaffin granules, number density, and frequency of spontaneous fusion or withdrawal into the cytoplasm. (5) Upon stimulation with high extracellular potassium, TIRFM reports depletion of the `visible pool' of vesicles closest to the plasma membrane within hundreds of milliseconds, consistent with previous concepts of a release-ready pool. We conclude that TIRFM constitutes an independent assay for pool depletion. TIRFM will allow us to study aspects of secretion that have previously been inaccessible in living cells, in particular the spatial relations and dynamics of vesicles prior to and during exocytosis and re-supply of the near-membrane pool of vesicles. Received: 26 June 1997 / Accepted: 26 September 1997     

A novel tight cylindrical mold for epoxy resin embedding allows enhanced microscopic analysis of microcores extracted from woody plants

A novel mold was devised to embed microcores extracted from stems of trees in epoxy resin, which has been widely used for optical and electron microscopic analysis of xylem formation. The embedding mold of a tight cylindrical shaped tube was designed to avoid displacement of microcores from the right position during the process of resin embedding. Microcores of a ring-porous hardwood species, Quercus crispula, with higher wood density and much larger differentiating vessel elements laid down on the boundary between the current xylem and the previous one, which generally cause difficulty in thin sectioning and breaks in sections, respectively, were embedded in the cylindrical molds full of epoxy resin. Locations of the three principal planes of wood anatomy could be determined in cylindrical resin-embedded microcores as follows: the transverse plane could be found on their side of cylinder, the radial one was vertical to the transverse, and the tangential ones were their circular ends of cylinder. The present embedding mold, therefore, can provide all three principal sections for microscopic wood anatomy from the side or ends of the same cylindrical microcore in principle. To confirm the usefulness of the resin-embedded microcores, we examined the differentiation of vessel elements during the period of earlywood formation on their transverse sections under microscopes, consequently could observe cell division in the cambial zone and sequential stages of vessel element differentiation, including cell expansion and deposition of the secondary cell wall. The present embedding mold for epoxy resin is simple but highly useful and innovative for a wide range of applications of microcores in microscopy for studies on tree-ring formation.     

水稻成熟花药和花粉的结构和组织化学研究

用乙二醇甲基丙烯酸脂(简称GMA)和环氧树脂Epon812包埋的薄切片方法对水稻成熟花药和花粉的结构进行了观察,并对各种结构的性质和细胞中的后含物做了细胞化学的分析.对成熟花药的绒毡层膜及乌氏体的研究采用了分离技术,做了显微和超微观察.证明水稻成熟花药壁和花粉除具一般禾本科植物特征外,还揭示了花药壁表皮上可能有硅质,药壁表皮细胞内含有脂类颗粒,药室内壁具纤维素质的纤维状加厚;发现花粉粒中除了贮存有大量淀粉颗粒外,还含有脂类,成熟花粉中营养核与两个精细胞及两个精细胞间联系紧密;并讨论了薄切片的优越性,绒毡层膜的意义及其上细胞印迹的来源.     

A Technical Perspective in Modern Tree-ring Research - How to Overcome Dendroecological and Wood Anatomical Challenges

Dendroecological research uses information stored in tree rings to understand how single trees and even entire forest ecosystems responded to environmental changes and to finally reconstruct such changes. This is done by analyzing growth variations back in time and correlating various plant-specific parameters to (for example) temperature records. Integrating wood anatomical parameters in these analyses would strengthen reconstructions, even down to intra-annual resolution. We therefore present a protocol on how to sample, prepare, and analyze wooden specimen for common macroscopic analyses, but also for subsequent microscopic analyses. Furthermore we introduce a potential solution for analyzing digital images generated from common small and large specimens to support time-series analyses. The protocol presents the basic steps as they currently can be used. Beyond this, there is an ongoing need for the improvement of existing techniques, and development of new techniques, to record and quantify past and ongoing environmental processes. Traditional wood anatomical research needs to be expanded to include ecological information to this field of research. This would support dendro-scientists who intend to analyze new parameters and develop new methodologies to understand the short and long term effects of specific environmental factors on the anatomy of woody plants.     

粗茎鳞毛蕨原叶体细胞有丝分裂过程中微管列阵的变化

应用Steedman‘s wax切片法,间接免疫荧光标记技术和激光共聚焦扫描显微镜技术研究了粗茎鳞毛蕨（Dryopteris crassirhizoma Nakai)原叶体大液泡化细胞和分生组织细胞有丝分裂过程中微管列阵的变化。结果显示：应用高浓度的多聚甲醛（8%）可以很好地保持大液泡化细胞的结构和微管的抗原性。结果也显示Steedman‘s wax切片法和间接免疫荧光标记技术的优点;（1）避免在微管标记过程中酶解细胞壁;（2）在乙醇脱水过程中样品中叶绿素的自发荧光被减到最小;（3）能够详细观察到有丝分裂过程中微管骨架的变化。因此,这种方法可以被广泛用来调查简单植物体和复杂植物体中细胞的有丝分裂过程以及发育过程中微管骨架的变化。