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培养获得的巨核细胞集落中倍性分布的测定:血小板减少症影响的研究

Measurement of ploidy distribution in megakaryocyte colonies obtained from culture: with studies of the effects of thrombocytopenia.

作者信息

Levin J, Levin F C, Penington D G, Metcalf D

出版信息

Blood. 1981 Feb;57(2):287-97.

PMID:7448424
Abstract

Microdensitometric measurement of the DNA content of individual megakaryocytes was performed using megakaryocyte colonies obtained following culture, in soft agar, of hematopoietic cells from C57BL/6J mice. Two types of colonies were detected. After 7 days of culture, the big cell type contained 16 /+- 2.3 acetylcholinesterase (AChE) positive cells/colony, with a mean ploidy level of 16.8 /+- 0.8/cell and the ploidy distribution characteristic of recognizable megakaryocytes in bone marrow. The heterogeneous type contained 44 /+- 9.6 cells/colony (some of which were AChE negative), with a mean ploidy level of 6.8 /+- 0.7/cell. The ploidy distribution of heterogeneous colonies differed markedly from big cell colonies, with preponderance of 2N and 4N cells. Colony-forming cells, obtained 4-5 days after induction of acute thrombocytopenia, gave big cell colonies with a marked increase in DNA content. Mean ploidy level increased to 21.5 /%- 1.8/cell; the frequency of 32N cells increased from 17% to 30% and 64N cells from 0% to 6%. This is the pattern of change observed in bone marrow, in vivo, 24 to 48 hr after induction of acute thrombocytopenia. The number of cells/colony did not increase. In contrast, acute thrombocytopenia did not alter the ploidy of heterogeneous colonies. The different responses to the stimulus of acute thrombocytopenia suggest that there are at least two types of Meg-CFC. The delayed appearance of altered Meg-CFC that produced big cell colonies indicates that the pool of stem cells, from which committed megakaryocyte precursors are derived, may respond indirectly to the stimulus of platelet depletion.

摘要

使用从C57BL/6J小鼠的造血细胞在软琼脂中培养后获得的巨核细胞集落,对单个巨核细胞的DNA含量进行了显微密度测定。检测到两种类型的集落。培养7天后,大细胞类型每个集落含有16±2.3个乙酰胆碱酯酶(AChE)阳性细胞,平均倍性水平为16.8±0.8/细胞,具有骨髓中可识别巨核细胞的倍性分布特征。异质类型每个集落含有44±9.6个细胞(其中一些为AChE阴性),平均倍性水平为6.8±0.7/细胞。异质集落的倍性分布与大细胞集落明显不同,以2N和4N细胞为主。在急性血小板减少症诱导后4-5天获得的集落形成细胞产生了DNA含量显著增加的大细胞集落。平均倍性水平增加到21.5±1.8/细胞;32N细胞的频率从17%增加到30%,64N细胞从0%增加到6%。这是在急性血小板减少症诱导后24至48小时在体内骨髓中观察到的变化模式。每个集落的细胞数量没有增加。相反,急性血小板减少症并未改变异质集落的倍性。对急性血小板减少症刺激的不同反应表明至少存在两种类型的巨核细胞集落形成细胞(Meg-CFC)。产生大细胞集落的Meg-CFC改变的延迟出现表明,从中产生定向巨核细胞前体的干细胞池可能对血小板减少的刺激产生间接反应。

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