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集落刺激活性在小鼠长期骨髓培养中的作用:贴壁细胞产生和消耗集落刺激活性的证据

Role of colony-stimulating activity in murine long-term bone marrow cultures: evidence for its production and consumption by the adherent cells.

作者信息

Heard J M, Fichelson S, Varet B

出版信息

Blood. 1982 Apr;59(4):761-7.

PMID:6977389
Abstract

The involvement of colony-stimulating activity (CSA) in murine long-term bone marrow cultures (LTBMC) was studied using bilayer agar cultures. The supernatants of LTBMC were removed, a layer of dense agar was spread over the cells adherent to the bottom of the flask, and fresh myeloid cells were plated as source of CFU-C in an upper agar layer. Large numbers of granulocytic and macrophagic colonies developed regularly when target cells were plated over adherent cells of nonrecharged and greater than 12 wk old LTBMC that were hematopoietically inactive (i.e., producing a low number of nonadherent cells). The removal of adherent cells from the myeloid cells used as source of CFU-C did not decrease the number of colonies. This suggests that adherent cells of LTBMC release CSA that is directly active on CFU-C. This CSA was no longer detectable over adherent layers of hematopoietically active LTBMC. A close inverse relationship was demonstrated between the number of nonadherent cells harvested before the assay and the level of CSA. No inhibitor for CSA was demonstrated in the supernatant of hematopoietically active cultures. Murine exogenous CSA incubated over the adherent layer host its activity within 24 hr, whereas in the same conditions human CSA retained its activity. These data demonstrate the production of CSA by the adherent layer of LTBMC and strongly suggest its specific in situ consumption by differentiating myeloid cells.

摘要

利用双层琼脂培养法研究了集落刺激活性(CSA)在小鼠长期骨髓培养(LTBMC)中的作用。去除LTBMC的上清液,在贴附于培养瓶底部的细胞上铺上一层致密琼脂,然后将新鲜的髓样细胞接种在上层琼脂层中作为CFU-C的来源。当将靶细胞接种在造血不活跃(即产生少量非贴壁细胞)的未再充能且大于12周龄的LTBMC的贴壁细胞上时,会定期形成大量粒细胞和巨噬细胞集落。从用作CFU-C来源的髓样细胞中去除贴壁细胞不会减少集落数量。这表明LTBMC的贴壁细胞释放出对CFU-C具有直接活性的CSA。在造血活跃的LTBMC的贴壁层上不再检测到这种CSA。在测定前收获的非贴壁细胞数量与CSA水平之间呈现密切的负相关关系。在造血活跃培养物的上清液中未发现CSA的抑制剂。将小鼠外源性CSA接种在贴壁层上,其活性在24小时内丧失,而在相同条件下,人CSA仍保持其活性。这些数据证明了LTBMC贴壁层产生CSA,并强烈提示其在髓样细胞分化过程中被特异性原位消耗。

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