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小鼠骨髓中的前B细胞:通过荧光激活细胞分选从骨髓中分离出的花生凝集素结合B淋巴细胞前体的体外成熟。

Pre-B cells in mouse bone marrow: in vitro maturation of peanut agglutinin binding B lymphocyte precursors separated from bone marrow by fluorescence-activated cell sorting.

作者信息

Osmond D G, Melchers F, Paige C J

出版信息

J Immunol. 1984 Jul;133(1):86-90.

PMID:6427348
Abstract

Peanut agglutinin (PNA) binding by mouse bone marrow cells and fractionation by the fluorescence-activated cell sorter have previously been shown to separate high concentrations of pre-B cells, as identified by cytoplasmic mu-chains (c mu). PNA+ and PNA- marrow cell fractions have now been assayed for the presence of functional pre-B cells able to generate mature B cells in culture, as defined by three criteria, the appearance of cell surface mu-chains (s mu), immunoglobulin secretion in response to bacterial lipopolysaccharides, and B cell colony formation. Small PNA+ cell fractions contained pre-B cells that developed into mature B lymphocytes in 1/2 to 1 day but did not sustain B cell production. Large PNA+ cells included pre-B cells that gave rise to mature B lymphocytes after an interval of 1 1/2 to 3 days and were able to sustain B cell genesis in vitro for at least 3 to 5 days thereafter. PNA- cell fractions contained mature B cells but lacked pre-B cell activity. The results demonstrate that PNA binding allows the separation of functional subsets of pre-B cells from bone marrow and that the three in vitro assays used in this study are closely comparable with one another as functional pre-B cell criteria. The findings suggest correlations between functional assays, c mu expression, PNA receptors, and cell size in characterizing stages of pre-B cell development.

摘要

先前已证明,通过小鼠骨髓细胞与花生凝集素(PNA)结合并利用荧光激活细胞分选仪进行分离,可以将高浓度的前B细胞分离出来,这些细胞可通过细胞质μ链(cμ)进行鉴定。现在,已对PNA +和PNA-骨髓细胞组分进行了检测,以确定是否存在能够在培养中产生成熟B细胞的功能性前B细胞,这通过三个标准来定义,即细胞表面μ链(sμ)的出现、对细菌脂多糖的免疫球蛋白分泌以及B细胞集落形成。小的PNA +细胞组分含有前B细胞,这些前B细胞在1/2到1天内发育成成熟的B淋巴细胞,但不能维持B细胞的产生。大的PNA +细胞包括前B细胞,这些前B细胞在1 1/2到3天的间隔后产生成熟的B淋巴细胞,并能够在体外维持B细胞发生至少3到5天。PNA-细胞组分含有成熟的B细胞,但缺乏前B细胞活性。结果表明,PNA结合可将骨髓中的功能性前B细胞亚群分离出来,并且本研究中使用的三种体外检测方法作为功能性前B细胞标准彼此具有高度可比性。这些发现表明,在表征前B细胞发育阶段时,功能检测、cμ表达、PNA受体和细胞大小之间存在相关性。

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