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首页> 外文期刊>Applied immunohistochemistry and molecular morphology: AIMM >Cell culture block array for immunocytochemical study of protein expression in cultured cells.
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Cell culture block array for immunocytochemical study of protein expression in cultured cells.

机译:细胞培养块阵列用于免疫细胞化学研究培养细胞中蛋白质的表达。

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摘要

Immunocytochemical staining of cultured cells using specific antibodies is a powerful technique to study the expression and subcellular localization of proteins. However, this technique is associated with sample-to-sample variations because samples are handled individually and manually. Cell permeation is needed when intracytoplasmic or nuclear proteins are studied. Storage of cultured cells is difficult, and experiments must be repeated if additional studies are desired later, which introduces more variations. We developed a cell culture block array technique that converts cultured cells into a permanently fixed form identical to tissue sections prepared for pathologic examination. Cells from different cultures can be embedded in a single block. Many identical sections, each containing cells from multiple cultures, may be stained with different antibodies using an automated stainer. As a result, sample-to-sample variation is eliminated. Because cells in these blocks are sectioned by knives, all cellular proteins come into direct contact with antibodies, and cell permeation is not needed. Such blocks can be conveniently stored for years without loss of antigens, providing a constant source for future studies. We demonstrated the utility of this technique by studying the proliferation and neuroendocrine differentiation of prostate cancer-derived LNCaP cells cultured in vitro.
机译:使用特异性抗体对培养细胞进行免疫细胞化学染色是研究蛋白质表达和亚细胞定位的强大技术。但是,由于样本是单独和手动处理的,因此该技术与样本之间的差异相关。研究细胞质或核蛋白时需要细胞渗透。培养的细胞很难保存,如果以后需要进行其他研究,则必须重复实验,这会引起更多的变化。我们开发了一种细胞培养块阵列技术,可将培养的细胞转变为与准备用于病理检查的组织切片相同的永久固定形式。可以将来自不同文化的细胞嵌入单个模块中。许多相同的切片,每个切片包含来自多个培养物的细胞,可以使用自动染色器用不同的抗体染色。结果,消除了样本之间的差异。由于这些区域中的细胞被刀具切开,因此所有细胞蛋白都直接与抗体接触,因此不需要细胞渗透。这样的块可以方便地保存数年而不会丢失抗原,为将来的研究提供了稳定的来源。我们通过研究体外培养的前列腺癌衍生的LNCaP细胞的增殖和神经内分泌分化,证明了该技术的实用性。

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