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Thiosemicarbazide used after periodic acid makes methenamine silver staining of renal glomerular basement membranes faster and cleaner. 经周期酸处理后使用硫代氨基脲可使肾小球基底膜甲基胺银染色更快、更干净。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106997
I Hayashi, Y Tome, Y Shimosato

The periodic acid-methenamine silver staining technique, which is frequently used for demonstrating the renal glomerular basement membrane, requires a high degree of skill, and in some cases it may be difficult to obtain a good result. To overcome such difficulty and inconsistency, we have improved the method by performing methenamine silver staining after oxidation with periodic acid and subsequent application of thiosemicarbazide. In this procedure, this semicarbazide enhanced the reaction of methenamine silver with the glomerular basement membrane and the reaction was completed within a shorter time in comparison with the conventional method. This modification also eliminated any nonspecific reaction with the surface of the glass slide and the solution container and yielded excellent and reproducible results irrespective of the fixation method and material employed. It was also found to stain the renal glomerular basement membrane of rabbits, which is demonstrable only with difficulty by the conventional method.

常用于肾小球基底膜显示的周期性酸-甲基苯丙胺银染色技术对技术要求较高,在某些情况下可能难以获得良好的结果。为了克服这种困难和不一致性,我们改进了方法,用周期酸氧化后进行甲基苯丙胺银染色,然后应用硫代氨基脲。在此过程中,氨基脲增强了甲基胺银与肾小球基底膜的反应,与常规方法相比,反应在更短的时间内完成。这种修饰还消除了与载玻片表面和溶液容器的任何非特异性反应,并且无论采用何种固定方法和材料,都产生了极好的可重复性结果。在家兔肾小球基底膜上也发现了染色,这是常规方法难以证实的。
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引用次数: 14
Fluorescence of plastic embedded tissue sections after curcumin staining. 姜黄素染色后塑料包埋组织切片的荧光。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909107001
J C Stockert, P Del Castillo, P S Testillano, M C Risueño
The natural dye, curcumin (C.I. 75300) from turmeric, is obtained from the roots of Curcuma longa (Lillie 1977). Curcumin has scarcely been applied for histological work, and its fluorescence seems to have been overlooked. During the course of studies on fluorescent aluminum complexes (Del Castillo et al. 1987) we realized that this dye induces a green fluorescence of chromatin (Stockert et al. 1989). In this note we describe the fluorescence reaction of curcumin on semithin sections of olastic embedded tissues.
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引用次数: 6
A simple method for staining nuclei of mature and germinated maize pollen. 成熟和发芽玉米花粉核染色的简单方法。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106996
M T Chang, M G Neuffer

A sugar acetocarmine staining technique has been developed for staining the sperm and vegetative nucleus of mature and germinated maize pollen grains. This procedure is simple, stable and highly repeatable. The physiological properties of the mature maize pollen grains are first adjusted by using an in vitro germinating culture solution. This solution is 15% sucrose and contains 360 ppm calcium chloride dihydrate, and 120 ppm boric acid. One part fresh pollen grains is uniformly mixed with nine parts of the solution and left at room temperature for at least 5 hr. One part of this solution is then mixed with two parts of regular acetocarmine stain and left overnight. The color of this mixture is pinkish red or raspberry. The sugar in the mixture helps to increase color contrast between the pollen cytoplasm (light pink) and the nuclei (reddish purple), decreases the frequency of burst pollen, increases pollen expansion, stabilizes pollen figures and automatically seals the coverglass.

建立了一种糖乙酰胭脂红染色技术,用于对成熟和萌发的玉米花粉粒的精子和营养核进行染色。该过程简单、稳定、可重复性高。首先利用离体萌发培养液调节成熟玉米花粉粒的生理特性。这个溶液是15%的蔗糖,含有360 ppm的氯化钙二水合物和120 ppm的硼酸。将一份新鲜花粉粒与九份溶液均匀混合,在室温下放置至少5小时。然后将该溶液的一部分与两份常规乙酰胭脂红染色剂混合并放置过夜。这种混合物的颜色是粉红色或覆盆子色。混合物中的糖有助于增加花粉细胞质(浅粉色)和细胞核(红紫色)之间的颜色对比,减少花粉破裂的频率,增加花粉膨胀,稳定花粉数量并自动密封盖玻璃。
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引用次数: 14
The ultramicrotome superstage: a versatile aid for section manipulation. 超微组超级级:一个多功能的辅助切片操作。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106999
M A Gorycki

The design and properties of a rigid, box-like device to be placed on the knife stage of a Porter-Blum MT-2 ultramicrotome are described. This "superstage" acts as a hand and tool rest, and a wind screen for the knife boat. The superstage easily permits tight rafts of ultrathin sections to be centrally located on grids. Additionally, it aids in placing 1 micron thick sections at the same relative location on glass slides to facilitate their examination in the light microscope.

描述了一种刚性的、盒状装置的设计和性能,该装置被放置在波特-布鲁姆MT-2微型手术刀台上。这个“超级舞台”充当手和工具架,以及刀船的挡风玻璃。超级级很容易允许超薄部分的紧筏位于网格的中央。此外,它有助于将1微米厚的切片放置在玻璃载玻片上的相同相对位置,以便于光显微镜下进行检查。
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引用次数: 0
A new method for preparation of undecalcified bone sections. 一种制备未钙化骨切片的新方法。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909107000
D L Sterchi, J A Eurell

A new method for preparation of sections of undecalcified bone is described. Samples of ovine bone were embedded in methylmethacrylate and thick-sectioned with a cutoff machine or commercial band saw. Composite slides were prepared by gluing white acrylic to glass using cyanoacrylate glue. Bone sections were glued to the composite slide and then surface polished by grinding or ultramilling. The polished surface of the section was then etched and stained. The techniques described in this paper reduce the time spent grinding or milling sections and improve resolution of surface-stained features of undecalcified bone sections.

介绍了一种制备非钙化骨切片的新方法。将羊骨样品包埋在甲基丙烯酸甲酯中,并用切断机或商用带锯进行厚切片。采用氰基丙烯酸酯胶将白色丙烯酸树脂粘接到玻璃上,制备复合玻片。骨段粘在复合载玻片上,然后通过研磨或超磨抛光表面。然后对该部分的抛光表面进行蚀刻和染色。本文描述的技术减少了研磨或研磨切片所花费的时间,并提高了未钙化骨切片表面染色特征的分辨率。
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引用次数: 29
Assessment of demyelination in glycol methacrylate sections: a new protocol for cresyl fast violet staining. 甲基丙烯酸乙二醇切片脱髓鞘的评估:甲酰耐紫外染色的新方案。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106993
K B Nguyen, M P Pender

A simple staining technique for nervous tissue is described. Tissue perfused with glutaraldehyde and formaldehyde and postfixed with osmium tetroxide is embedded in glycol methacrylate. One-micrometer sections are stained with 0.05% cresyl fast violet aqueous solution at 60 C for 5 min, washed with tap water and air dried. With this method the details of all nervous tissue elements are clearly demonstrated. The technique is particularly useful for assessing demyelination because the staining of axoplasm allows demyelinated axons to be well visualized.

描述了一种简单的神经组织染色技术。用戊二醛和甲醛灌注组织,用四氧化锇后固定,包埋在甲基丙烯酸乙二醇酯中。1微米切片用0.05%甲酚耐晒紫水溶液在60℃下染色5分钟,用自来水洗涤,风干。用这种方法可以清楚地显示所有神经组织元素的细节。该技术对评估脱髓鞘特别有用,因为轴质染色可以很好地显示脱髓鞘轴突。
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引用次数: 13
High resolution techniques for study of human centromeric heterochromatin. 人类着丝异染色质研究的高分辨率技术。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106994
L Sanchez, V Goyanes

A high resolution procedure for analyzing human centromeric heterochromatin is described. The combined use of decondensation agents of pericentromeric heterochromatin and electron microscopy of whole mounted chromosomes allows a more precise identification of centromere and pericentromeric regions.

描述了一种分析人类着丝性异染色质的高分辨率方法。结合使用着丝粒周围异染色质的去浓缩剂和整个安装的染色体的电子显微镜可以更精确地识别着丝粒和着丝粒区域。
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引用次数: 3
Optimal parameters for the histochemical demonstration of acetylcholinesterase in plastic sections of rat brain. 大鼠脑塑料切片乙酰胆碱酯酶组织化学研究的最佳参数。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106995
L R Williams, M R Donald, K S Jodelis

A modified method for improved preservation and optical resolution of acetylcholinesterase (AChE)-containing structures in adult rat brain is described. Optimal tissue preparation included fixation in paraformaldehyde 4%, glutaraldehyde 0.1%, and sucrose 7% in 0.1M Sorensen's phosphate buffer, pH 7.4, rinsing in buffer 50 mM with respect to NH4Cl and 2% with respect to sucrose, acetone dehydration, vacuum infiltration with LKB Historesin, and polymerization at 4 C, overnight incubation of 10 microns sections at 37 C in the AChE histochemical reaction mixture and silver intensification according to Hedreen et al. Demonstration of AChE enzyme activity in the cholinergic projection from the rat basal forebrain to the ipsilateral hippocampus exemplifies the usefulness of the technique. The method provides an excellent demonstration of AChE-positive axonal processes and enables the pharmacohistochemical visualization of cholinergic neurons. This procedure offers a convenient method for analysis of cholinergic neurons that avoids potential artifacts inherent in other AChE histochemical procedures.

描述了一种改进的方法,以提高保存和光学分辨率的乙酰胆碱酯酶(AChE)在成年大鼠脑结构。根据Hedreen等人的研究,最佳组织制备方法为:在0.1M Sorensen磷酸缓冲液中,用4%的多聚甲醛、0.1%的glutaraldehyde和7%的蔗糖固定,pH为7.4,用50 mM的NH4Cl和2%的蔗糖在缓冲液中冲洗,丙酮脱水,用LKB组织树脂真空浸润,在4℃下聚合,在37℃下将10微米的片段在AChE组织化学反应混合物中过夜,并进行银强化。从大鼠基底前脑到同侧海马的胆碱能投射中乙酰胆碱酯酶的活性证明了该技术的有效性。该方法提供了ache阳性轴突过程的良好演示,并使胆碱能神经元的药物组织化学可视化成为可能。该程序为胆碱能神经元的分析提供了一种方便的方法,避免了其他乙酰胆碱酯酶组织化学程序中固有的潜在伪影。
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引用次数: 2
The use of gold chloride to stain developing and adult neuromuscular junctions in the insect. 用氯化金染色昆虫发育中的和成体的神经肌肉连接处。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106992
M B Rheuben, P J Schaner

Individual insect muscle fibers, whose neuromuscular junctions have been stained with a modification of Ranvier's gold chloride method, can be dissected free and mounted whole if the muscle is prefixed in aldehydes. The neuromuscular junctions along the length of the individual fibers are well delineated and can be measured and counted. Effective procedures include fixation with glutaraldehyde buffered to low pH with sodium citrate, or glutaraldehyde and paraformaldehyde combined in phosphate buffer at neutral pH, followed by exposure to citric acid and to gold chloride. The method is convenient, and could be useful for the study of arthropod neuromuscular junctions in general, since their nerve terminals do not release acetylcholine as a transmitter and cannot be stained by the more commonly used cholinesterase methods.

单个昆虫的肌肉纤维,其神经肌肉连接处已经用一种改进的兰维尔氯化金方法染色,如果在肌肉上加上醛,就可以自由地解剖和安装整个肌肉。沿着单个纤维的长度的神经肌肉连接被很好地描绘出来,并且可以被测量和计数。有效的方法包括用柠檬酸钠缓冲至低pH的戊二醛固定,或在中性pH下将戊二醛和多聚甲醛混合在磷酸盐缓冲液中固定,然后暴露于柠檬酸和氯化金。由于节肢动物的神经末梢不释放乙酰胆碱作为一种递质,而且不能被更常用的胆碱酯酶染色,因此该方法很方便,可用于一般节肢动物神经肌肉连接的研究。
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引用次数: 2
Hoechst 33342 staining coupled with conventional histological technique. Hoechst 33342染色结合常规组织学技术。
Pub Date : 1989-07-01 DOI: 10.3109/10520298909106998
W Sawicki, S Moskalewski

Hoechst 33342 was injected either intravenously or intraperitoneally into mice which were killed 1 or 24 hr or 7, 14 or 28 days later. Various organs were fixed and paraffin embedded. Visual inspection showed that independently of the route of dye administration or survival time, distinct fluorescence of nuclei was observed in organs other than cerebral cortex. Even formic acid decalcification of bone failed to abolish the fluorescence of osteocytes. In vivo staining with Hoechst 33342 is proposed as an alternative for staining after sectioning. Cells from spleens of Hoechst 33342-injected mice or stained in vitro were injected intramuscularly into mice. Hoechst 33342-stained splenocytes could be found in deparaffinized sections at the site of injection 24 hr later.

将Hoechst 33342分别静脉或腹腔注射到小鼠体内,分别于1、24小时或7、14、28天后死亡。固定各脏器,石蜡包埋。肉眼观察显示,与给药途径或存活时间无关,除大脑皮层外,其他器官均可见明显的细胞核荧光。即使甲酸脱钙也不能消除骨细胞的荧光。建议用Hoechst 33342进行体内染色,作为切片后染色的替代方法。取Hoechst 33342小鼠脾细胞肌内注射或体外染色。24小时后,在注射部位脱胶切片上可见Hoechst 33342染色的脾细胞。
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引用次数: 13
期刊
Stain technology
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