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正常和肿瘤性人B淋巴细胞产生集落刺激活性。

Production of colony-stimulating activity by normal and neoplastic human B lymphocytes.

作者信息

Pistoia V, Ghio R, Roncella S, Cozzolino F, Zupo S, Ferrarini M

出版信息

Blood. 1987 May;69(5):1340-7.

PMID:3494479
Abstract

Normal human B cells were purified from peripheral blood or tonsils and tested for their ability to release colony-stimulating activity (CSA) in short-term cultures. The target cells used in the CSA assays were from peripheral blood or bone marrow. Unstimulated B cells produced CSA in amounts similar to those present in the GCT-conditioned medium used as a positive control. The B cell-derived CSA predominantly promoted the growth of colonies that contained macrophages alone or macrophages and granulocytes. CSA eluted in a single peak from a G-75 Sephadex column with an approximate molecular weight (mw) of 65 to 70 kilodaltons (kd). Fractionation of tonsil B lymphocytes on Percoll density gradients showed that large B cells, probably already activated in vivo, were the main source of CSA. By contrast, small, resting B cells recovered from a different fraction of the Percoll gradient released minimum amounts or no CSA. However, these B cells became CSA producers following stimulation with Staphylococcus aureus Cowan (SAC) in vitro. B cells purified from the peripheral blood of nine out of 12 patients with B-cell chronic lymphocytic leukemia (B-CLL) also released CSA in vitro in the absence of stimuli. These findings suggest that by releasing CSA, B cells may have a role in the regulation of hematopoiesis and in the control of the inflammatory process.

摘要

从外周血或扁桃体中纯化正常人B细胞,并检测其在短期培养中释放集落刺激活性(CSA)的能力。CSA检测中使用的靶细胞来自外周血或骨髓。未刺激的B细胞产生的CSA量与用作阳性对照的GCT条件培养基中的量相似。B细胞衍生的CSA主要促进仅含有巨噬细胞或巨噬细胞和粒细胞的集落生长。CSA从G-75 Sephadex柱上以单一峰洗脱,其近似分子量(mw)为65至70千道尔顿(kd)。在Percoll密度梯度上对扁桃体B淋巴细胞进行分级分离表明,大B细胞可能已在体内被激活,是CSA的主要来源。相比之下,从Percoll梯度的不同部分回收的小的静止B细胞释放的CSA量最少或不释放CSA。然而,这些B细胞在体外经金黄色葡萄球菌Cowan株(SAC)刺激后成为CSA产生细胞。从12例B细胞慢性淋巴细胞白血病(B-CLL)患者中的9例患者的外周血中纯化的B细胞在无刺激的情况下也在体外释放CSA。这些发现表明,通过释放CSA,B细胞可能在造血调节和炎症过程控制中发挥作用。

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