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整合拉曼和角散射显微镜揭示了激活和未激活的 CD8+T 淋巴细胞之间的化学和形态差异。

Integrated Raman and angular scattering microscopy reveals chemical and morphological differences between activated and nonactivated CD8+ T lymphocytes.

机构信息

University of Rochester, The Institute of Optics, 275 Hutchison Road, Rochester, New York 14627, USA.

出版信息

J Biomed Opt. 2010 May-Jun;15(3):036021. doi: 10.1117/1.3443794.

Abstract

Integrated Raman and angular-scattering microscopy (IRAM) is a multimodal platform capable of noninvasively probing both the chemistry and morphology of a single cell without prior labeling. Using this system, we are able to detect activation-dependent changes in the Raman and elastic-scattering signals from CD8+ T cells stimulated with either Staphylococcal enterotoxin B (SEB) or phorbol myristate acetate (PMA). In both cases, results obtained from the IRAM instrument correlate well with results obtained from traditional fluorescence-based flow cytometry for paired samples. SEB-mediated activation was distinguished from resting state in CD8+ T cells by an increase in the number and mean size of small ( approximately 500-nm) elastic scatterers as well as a decrease in Raman bands, indicating changes in nuclear content. PMA-mediated activation induced a different profile in CD8+ T cells from SEB, showing a similar increase in small elastic scatterers but a different Raman change, with elevation of cellular protein and lipid bands. These results suggest the potential of this multimodal, label-free optical technique for studying processes in single cells.

摘要

集成拉曼和角散射显微镜(IRAM)是一种多模态平台,能够在无需预先标记的情况下非侵入性地探测单个细胞的化学和形态。使用该系统,我们能够检测到用葡萄球菌肠毒素 B(SEB)或佛波醇肉豆蔻酸酯(PMA)刺激的 CD8+ T 细胞的拉曼和弹性散射信号的激活依赖性变化。在这两种情况下,从 IRAM 仪器获得的结果与传统基于荧光的流式细胞术对配对样本的结果很好地相关。SEB 介导的激活与 CD8+ T 细胞的静息状态区分开来,这是通过小(约 500nm)弹性散射体的数量和平均尺寸的增加以及拉曼带的减少来指示核内容的变化。PMA 介导的激活在 CD8+ T 细胞中诱导与 SEB 不同的谱,显示出类似的小弹性散射体增加,但拉曼变化不同,细胞蛋白和脂质带升高。这些结果表明,这种多模态、无标记的光学技术在研究单个细胞中的过程具有潜力。

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