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通过连续的体内溴脱氧胞苷标记和流式细胞术分析研究小鼠骨髓、胸腺和脾脏中的细胞增殖。

Cell proliferation in the bone marrow, thymus and spleen of mice studied by continuous, in vivo bromodeoxycytidine labelling and flow cytometric analysis.

作者信息

Crippen T L, Jones I M

机构信息

Lawrence Livermore National Laboratory, Livermore, CA 94550.

出版信息

Cell Tissue Kinet. 1989 May;22(3):203-12. doi: 10.1111/j.1365-2184.1989.tb00206.x.

Abstract

We have applied the technique of labelling dividing cells with bromodeoxyuridine (BrdUrd) in combination with in vivo continuous labelling, propidium iodide (PI) staining for DNA content, and flow cytometric analysis, for the determination of cell proliferation in bone marrow, thymus and spleen of mice. The percentage of BrdUrd labelled cells increased as a function of exposure time in a tissue specific manner for each of the three tissues. Thymus and bone marrow had cell populations which exhibited different kinetics for the accumulation of label: (1) those that cycled and became labelled within 2-3 days (88% in 2 days for bone marrow, 84% in 3 days for thymus); (2) those that cycled during the remainder of the 6 day infusion period (11% of bone marrow and 13% of thymus cells); and (3) those that did not cycle during the 6 day period studied (less than 2% of bone marrow and 3% of thymus cells). In contrast, the spleen exhibited a slower, constant accumulation of labelled cells. After six days of infusion a large proportion of spleen cells (50%) had not become labelled. These results suggest that a larger proportion of spleen cells are long lived than indicated by other methods. We also have found the period of labelling with BrdUrd extended several days beyond the period of infusion. This method will be very useful in studying perturbations of cell populations induced in mice exposed to toxic agents.

摘要

我们应用了用溴脱氧尿苷(BrdUrd)标记分裂细胞的技术,并结合体内连续标记、碘化丙啶(PI)染色以测定DNA含量以及流式细胞术分析,来确定小鼠骨髓、胸腺和脾脏中的细胞增殖情况。在这三种组织中,BrdUrd标记细胞的百分比随暴露时间以组织特异性方式增加。胸腺和骨髓中有一些细胞群体,它们标记积累的动力学不同:(1)那些在2 - 3天内循环并被标记的细胞(骨髓中2天内为88%,胸腺中3天内为84%);(2)那些在6天输注期的剩余时间内循环的细胞(骨髓细胞的11%和胸腺细胞的13%);以及(3)那些在研究的6天期间不循环的细胞(骨髓细胞少于2%,胸腺细胞为3%)。相比之下,脾脏中标记细胞的积累较慢且持续。输注6天后,很大一部分脾细胞(50%)尚未被标记。这些结果表明,与其他方法所示相比,脾细胞中长寿细胞的比例更大。我们还发现用BrdUrd标记的时间比输注期延长了几天。这种方法在研究暴露于有毒物质的小鼠中诱导的细胞群体扰动方面将非常有用。

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