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A fast method to study the secretory activity of neuroendocrine cells at the ultrastructural level.

机译:在超微结构水平研究神经内分泌细胞分泌活性的快速方法。

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Summary Cryo field emission scanning electron microscopy (cryo-FE-SEM) is a versatile technique that allows the investigation of the three-dimensional organization of cells at the ultrastructural level over a wide range of magnifications. Unfortunately, cryopreparation of the specimens for this technique remains cumbersome, in particular because ice crystal formation must be prevented during freezing. Here we report that a light prefixation with glutaraldehyde and incubation in glycerol as cryoprotectant or a high-pressure freezing approach are both excellent procedures for cryopreparation of animal cells to be used in combination with cryo-FE-SEM. Using the proopiomelanocortin-producing intermediate pituitary melanotrope cells of Xenopus laevis as a physiologically inducible neuroendocrine system, we compared the ultrastructural characteristics of inactive and hyperactive neuroendocrine cells. The overall quality of the ultrastructural images was comparable for the two cryopreparation procedures, although some fine structures were better conserved using high-pressure freezing. Melanotrope cells in a secretory inactive state contained numerous storage granules and a poorly developed endoplasmic reticulum (ER), while large amounts of rough ER were present in hyperactive cells. Thus, the cryo-FE-SEM approach described here allows a fast ultrastructural study on the secretory activity of neuroendocrine cells.
机译:总结低温场发射扫描电子显微镜(cryo-FE-SEM)是一种通用技术,可用于在大范围放大倍率下研究超微结构水平细胞的三维组织。不幸的是,用于该技术的标本的冷冻修复仍然很麻烦,特别是因为在冷冻期间必须防止冰晶形成。在这里,我们报道了以戊二醛为光的前缀以及在甘油中作为冷冻保护剂或高压冷冻方法的孵育都是将动物细胞与冷冻-FE-SEM结合使用的低温修复的优秀方法。使用非洲爪蟾的产proopiomelanocortin的中间垂体黑素细胞作为生理上可诱导的神经内分泌系统,我们比较了无活性和高活性神经内分泌细胞的超微结构特征。尽管使用高压冷冻法可以更好地保存一些精细结构,但两种冷冻修复程序的超微结构图像的整体质量是可比的。处于分泌性失活状态的黑皮膜细胞含有许多储存颗粒和发育不良的内质网(ER),而在过度活跃的细胞中则存在大量的粗糙ER。因此,这里描述的cryo-FE-SEM方法可以对神经内分泌细胞的分泌活性进行快速的超微结构研究。

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