共查询到20条相似文献,搜索用时 15 毫秒
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Scanning and transmission electron microscopy of the rat kidney 总被引:2,自引:0,他引:2
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Scanning and transmission electron microscopy was applied for a morphological study of three strains of Bifidobacterium grown on solid or liquid media. The pronounced pleomorphism of the cultures previously observed by light microscopy was confirmed. A possible sequence of the morphological events during transformation from one to another pleomorphic form is proposed for B. bifidum and B. longum. Ultrastructural differences such as the formation of extensive mesosomal complexes in B. longum and characteristic plasmalemma particles only observed in the B. bifidum mutant are described and discussed. 相似文献
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C A Speer A A Marchiondo B Mueller D W Duszynski 《Zeitschrift für Parasitenkunde (Berlin, Germany)》1979,59(3):219-225
The oocyst wall of Isospora lacazei from sparrows was studied with scanning (SEM) and transmission (TEM) electron microscopy. In TEM, the oocyst wall consisted of four distinct layers (L1-4). The innermost layer, L1, was moderately electron-lucent and 240--285 nm thick; L2 was electron-dense and 210--240 nm thick; L3 was moderately electron-lucent and 15--150 nm thick; L4, the outer most layer, was discontinuous and consisted of electron-dense discoid bodies which measured 180--220 nm x 320--840 nm. The discoid bodies of L4 as seen by TEM appeared spheroid in shape when observed by SEM. One or two membranes were situated on or between various layers of the oocyst wall. One such membrane occurred on the inner margin of L1, two closely applied membranes were interposed between L1 and L2, one membrane occurred between L2 and L3, and one membrane on the outer margin of L3. 相似文献
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The exine stereostructure (scanning electron microscopy) and ultrastructure (transmission electron microscopy) of pollen of seven grass species, is related to the allergens extracted from these pollen grains. The heterogeneity of the allergens was studied by the immunoprint technique and revealed by labelling the binding of grass pollen sensitive patients IgE antibodies. Using patient sera recognizing a very restricted number of allergens, we showed that a group of pollen had a great number of allergens in common (Dactylis, Agrostis, Festuca, Lolium, Holcus) and, in decreasing cross reactivities order, we found Avena and, finally, Zea mays. The tectum stereostructure shows presence of insulae in all pollen grains except in Zea mays which has small isolated spinules. These insulae are separated by very wide and deep interinsular spaces in Avena sativa with connections between insulae. In the remaining species, no connections were seen between the insulae. These observations were in good correlation with the immunological cross-reactivity of the allergens present in the pollen. In all species, there are microperforations in the bottom of the interinsular spaces, which are the opening of the tectal microchannels. 相似文献
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Scanning electron microscopy of Drosophila 总被引:2,自引:0,他引:2
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Taupin P 《European journal of histochemistry : EJH》2008,52(2):135-139
Light microscopy (LM) and transmission electron microscopy (TEM) aim at understanding the relationship structure-function. With advances in biology, isolation and purification of scarce populations of cells or subcellular structures may not lead to enough biological material, for processing for LM and TEM. A protocol for preparation of scarce biological samples is presented. It is based on pre-embedding the biological samples, suspensions or pellets, in bovine serum albumin (BSA) and bis-acrylamide (BA), cross-linked and polymerized. This preparation provides a simple and reproducible technique to process biological materials, present in limited quantities that can not be amplified, for light and transmission electron microscopy. 相似文献
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Arterial repair after microvascular anastomosis. Scanning and transmission electron microscopy study
G Macchiarelli G Familiari A Caggiati F M Magliocca F Riccardelli A Miani P M Motta 《Acta anatomica》1991,140(1):8-16
In order to study the morphological aspects of endothelial regeneration and vascular wall reaction after microvascular anastomosis, rat femoral arteries were sectioned and successively sutured (end-to-end anastomosis) with microsurgical techniques. Control arteries and anastomosed vessels (recovered after 1, 4, 7, 14, 21, 30, 60, 120, 180 and 360 days) were studied by means of scanning (SEM) and transmission electron microscopy (TEM). The reendothelialization phenomena started after 7 days and were mainly evident at 21 days. Areas of subendothelial connective tissue with fibrin deposition remained exposed to the blood stream up to 21-30 days. Thrombus formations or post-anastomotic stenosis have been occasionally observed. Regenerating endothelium showed evident morphological differences from the control. These changes mainly consisted of shortened cell length, absence of pinocytotic vesicles, presence of cytoplasmic prolongations, and microvillous proliferations. The arterial wall showed subintimal thickening. The anastomotic site appeared completely covered by new endothelium after 30-60 days. Subintimal vascular wall changes (thickening of the media) as well as slight alterations of endothelial cells (shortened length, reduced number of pinocytotic vesicles) were evident in 60-day vessels. Lumen reduction, due to the protruding of endothelial-covered sutures, was occasionally observed in 60- to 120-day arteries. Endothelial cell morphology normalized after 60-120 days. However, thickening of the media and occasional lumen reduction were observed also after 180-360 days. Although the endothelial regeneration phenomena were clearly evident after 2 weeks, nevertheless the reestablishment of arterial wall took longer time.(ABSTRACT TRUNCATED AT 250 WORDS) 相似文献
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The scanning transmission electron microscope (STEM) is discussed in view of biological applications. Theoretical considerations are given, but the emphasis is directed to practical examples from a range of biological projects. The STEM is most efficiently used in elastic and inelastic dark-field modes providing information on the scattering power of the irradiated sample. Thus, the STEM is an ideal tool for quantitative measurements such as mass-mapping or element-mapping at high resolution. Limitations of such methods due to multiple scattering and quantum noise are briefly reviewed. 相似文献
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The morphology of conidia in 211 species and 12 varieties belonging to the genus Penicillium Link ex Gray have been studied and compared.According to surface ornamentation, conidia have been classified into six groups: A, smooth-walled (7% of the species); B, delicately roughened (13%); C, warty (28%); D, echinate (10%); E, striate with low irregular ridges (36%); and F, striate with scarce high ridges or bars (6%). Whereas the first two groups are closely related in both shape and average size, a gradual reduction was observed in size and in the length/width (l/w) ratio in the remaining groups. Echinate conidia were globose, having the largest average size. Only four species produced conidia not surpassing 2 m in diameter. Maximum length observed was 8 m, and most elongated conidia had a l/w ratio of 3.5. Forty per cent of the species studied had globose conidia.Conidia of the monoverticillate species were generally smaller, more globose and frequently with ridges. In the Asymmetrica, the conidia were generally larger, and showed ridges in comparatively few species. Conidia of the Symmetrica, which were frequently striate with ridges, presented the most elongated forms. The largest average size was found in the conidia of the Polyverticillata which were generally warty. Finally, we have considered the variations in surface ornamentation of conidia during the evolution of the genus Penicillium and drawn attention to their possible relationship with certain habitats and ways of conidial dispersion. 相似文献
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Mark Winey Janet B. Meehl Eileen T. O'Toole Thomas H. Giddings Jr. 《Molecular biology of the cell》2014,25(3):319-323
Researchers have used transmission electron microscopy (TEM) to make contributions to
cell biology for well over 50 years, and TEM continues to be an important technology in
our field. We briefly present for the neophyte the components of a TEM-based study,
beginning with sample preparation through imaging of the samples. We point out the
limitations of TEM and issues to be considered during experimental design. Advanced
electron microscopy techniques are listed as well. Finally, we point potential new users
of TEM to resources to help launch their project.Transmission electron microscopy (TEM) has been an important technology in cell biology ever
since it was first used in the early 1940s. The most frequently used TEM application in cell
biology entails imaging stained thin sections of plastic-embedded cells by passage of an
electron beam through the sample such that the beam will be absorbed and scattered, producing
contrast and an image (see Term Definition Beem capsule Plastic forms that hold samples in resin during polymerization Blocks (bullets) Polymerized samples in plastic removed from the Beem capsule and ready
to section Block face Small surface trimmed on a block before sectioning Boat Water reservoir in which sections float after being cut by a knife CLEM Correlative light and electron microscopy Dehydration Removal of water from a sample by replacement with solvent Electron tomography (ET) A method to image thick sections (200–300 nm) and produce
three-dimensional images Embedding Process of infiltrating the sample with resin Fixation Sample preservation with low temperature and/or chemicals to maintain
sample integrity Grid Small metal support that holds the sections for viewing in the electron
microscope HPF/FS High-pressure freezing/freeze substitution sample preparation
technique Immuno-EM Detection of proteins in EM samples using antibodies In-FXXKing credible!!!! Actual user quote in response to particularly beautiful sample. You may
embellish with your own words. Knife A very sharp edge, either glass or diamond, used to slice off
resin-embedded samples into sections Pre-embedding labeling Application of antibodies before fixation and embedding Post-embedding labeling Application of antibodies to sections on the grid Poststaining Staining with heavy metals of sections on a grid Resin Liquid form of the plastics used for embedding Ribbon Collection of serial sections placed on the grid Serials sections One-after-the-other thin sections in a ribbon TEM Transmission electron microscopy Thin sections The 60- to 70-nm sections cut from the samples in blocks Trimming Process of cutting away excess resin to create a block face Ultramicrotome Instrument used to cut sections Vitrification/vitreous ice Unordered ice in which samples can be viewed without fix or stain