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首页> 外文期刊>Microscopy and microanalysis: The official journal of Microscopy Society of America, Microbeam Analysis Society, Microscopical Society of Canada >Processing Techniques for Scanning Electron Microscopy Imaging of Giant Cells from Giant Cell Tumors of Bone
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Processing Techniques for Scanning Electron Microscopy Imaging of Giant Cells from Giant Cell Tumors of Bone

机译:从骨巨细胞肿瘤扫描巨细胞电子显微镜成像的处理技术

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摘要

Giant cell tumor (GCT) of bone is a common benign lesion that causes significant morbidity due to the failure of modern medical and surgical treatment. Surface ultra-structures of giant cells (GCs) may help in distinguishing aggressive tumors from indolent GC lesions. This study aimed to standardize scanning electron microscopic (SEM) imaging of GC from GCT of bone. Fresh GCT collected in Dulbecco's Modified Eagle Medium was washed to remove blood, homogenized, or treated with collagenase to isolate the GCs. Mechanically homogenized and collagenase-digested GCs were imaged on SEM after commonly used drying methodologies such as air-drying, tetramethylsilane (TMS)-drying, freeze-drying, and critical point-drying (CPD) for the optimization of sample processing. The collagenase-treated samples yielded a greater number of isolated GC and showed better surface morphology in comparison to mechanical homogenization. Air-drying was associated with marked cell shrinkage, and freeze-dried samples showed severe cell damage. TMS methodology partially preserved the cell contour and surface structures, although the cell shape was distorted. GC images with optimum surface morphology including membrane folding and microvesicular structures on the surface were observed only in collagenase-treated and critical point-dried samples. Collagenase digestion and critical point/TMS-drying should be performed for optimal SEM imaging of individual GCs.
机译:骨的巨细胞肿瘤(GCT)是一种常见的良性病变,由于现代医学和手术治疗的失败导致显着的发病率。巨细胞(GCS)的表面超结构可以有助于区分来自惰性GC病变的侵袭性肿瘤。本研究旨在标准骨骼GCT的扫描电子显微镜(SEM)成像。在Dulbecco的改性鹰培养基中收集的新鲜GCT洗涤以除去血液,均质化或用胶原酶处理,以分离GCS。在常用的干燥方法之后的SEM上在诸如风干,四甲基硅烷(TMS) - 加热,冷冻干燥和临界点干燥(CPD)之后的SEM上成像在SEM上进行成像,用于优化样品处理。与机械均化相比,胶原酶处理的样品产生更多的分离的GC,并且显示出更好的表面形态。风干与显着的细胞收缩相关,冷冻干燥的样品显示出严重的细胞损伤。 TMS方法部分保留了细胞轮廓和表面结构,尽管细胞形状扭曲。仅在胶原酶处理和临界点干燥的样品中观察到具有膜折叠和表面上的微孔结构的最佳表面形态的GC图像。应对胶原酶消化和临界点/ TMS干燥进行各个GCS的最佳SEM成像。

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