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大鼠骨髓细胞培养中树突状细胞的分化

Differentiation of dendritic cells in cultures of rat bone marrow cells.

作者信息

Bowers W E, Berkowitz M R

出版信息

J Exp Med. 1986 Apr 1;163(4):872-83. doi: 10.1084/jem.163.4.872.

Abstract

Although dendritic cells (DC) originate from bone marrow, they were not observed in fresh preparations of bone marrow cells (BMC). Likewise, accessory activity was barely measurable in a sensitive assay for this potent function of DC. However, both DC and accessory activity developed when BMC were cultured for 5 d. Based on fractionation before culture, nearly all of the accessory activity could be attributed to only 5% of the total BMC recovered in a low-density (LD) fraction. The LD-DC precursors differed from mature DC in a number of important respects. Removal of Ia+ cells from the LD fraction by panning did not decrease the production of DC when the nonadherent cells were cultured. Thus, the cell from which the DC is derived does not express or minimally expresses Ia antigens, in contrast to the strongly Ia+ DC that is produced in bone marrow cultures. Irradiation of LD cells before culture prevented the development of DC. When irradiation was delayed by daily intervals, progressive increases in the number of DC resulted, up to the fifth day. These findings, together with preliminary autoradiographic data, indicate that cell division has occurred, in contrast to the DC, which does not divide. We conclude that bone marrow-derived DC arise in culture from the division of LD, Ia- precursors.

摘要

尽管树突状细胞(DC)起源于骨髓,但在新鲜的骨髓细胞(BMC)制剂中并未观察到它们。同样,在针对DC这种强大功能的灵敏检测中,辅助活性几乎无法测量。然而,当BMC培养5天时,DC和辅助活性都出现了。基于培养前的分级分离,几乎所有的辅助活性都仅归因于在低密度(LD)组分中回收的总BMC的5%。LD-DC前体在许多重要方面与成熟DC不同。通过淘选从LD组分中去除Ia⁺细胞,当非贴壁细胞培养时,DC的产生并未减少。因此,与骨髓培养中产生的强Ia⁺ DC相反,DC所源自的细胞不表达或极少表达Ia抗原。培养前对LD细胞进行照射可阻止DC的发育。当照射按日间隔延迟时,DC数量逐渐增加,直至第五天。这些发现,连同初步的放射自显影数据表明,与不分裂的DC相反,已经发生了细胞分裂。我们得出结论,骨髓来源的DC在培养中源自LD、Ia⁻前体的分裂。

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