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二磷酸腺苷对培养的造血细胞系的刺激作用。

Adenosine diphosphate stimulation of cultured hematopoietic cell lines.

作者信息

Kalambakas S A, Robertson F M, O'Connell S M, Sinha S, Vishnupad K, Karp G I

机构信息

Department of Medicine, UMDNJ-Robert Wood Johnson Medical School, New Brunswick 08903-0019.

出版信息

Blood. 1993 May 15;81(10):2652-7.

PMID:8490174
Abstract

Adenosine diphosphate (ADP) plays a critical role in platelet activation both by exogenous stimulation and the release of endogenous intracellular stores. As the platelet ADP receptor is not well defined, we have chosen to identify and characterize several cell lines that possess functional receptors for this nucleotide. Rat promegakaryoblasts (RPM), human erythroleukemia cells (HEL), U937, and K562 leukemia cells responded to ADP, as measured by a rapid increase in intracellular calcium. In the case of RPM cells, ADP was the only naturally occurring platelet agonist capable of eliciting this response. Binding studies with [3H]ADP and fixed cells showed 3.99 +/- 1.77 x 10(5) binding sites/cell for RPM cells (apparent dissociation constant [kd] = 7.75 +/- 2.3 x 10(-8) mol/L), 8.19 +/- 3.25 x 10(5) sites/cell for HEL cells (kd = 2.15 +/- 0.84 x 10(-7) mol/L, 1.15 +/- 0.23 x 10(6) sites/cell for U937 cells (kd = 2.20 +/- 0.53 x 10(-7) mol/L) and 5.39 +/- 2.80 x 10(5) sites/cell for K562 cells (kd = 1.37 +/- 0.39 x 10(-7) mol/L), Inhibition studies with unlabeled nucleotides and analogues showed that binding was approximately 85% specific and the inhibitory pattern was similar to that seen with mature platelets. The purine base adenosine resulted in little or no inhibition. These studies indicate that both human and rat hematopoietic cell lines possess intact ADP receptors and may be useful tools in future studies of the structure and function of this important platelet-activation system.

摘要

二磷酸腺苷(ADP)在外源性刺激和内源性细胞内储存物质释放过程中,对血小板激活均起着关键作用。由于血小板ADP受体尚未明确界定,我们选择鉴定和表征几种对该核苷酸具有功能性受体的细胞系。大鼠早幼巨核细胞(RPM)、人红白血病细胞(HEL)、U937和K562白血病细胞对ADP有反应,通过细胞内钙的快速增加来衡量。就RPM细胞而言,ADP是唯一能够引发这种反应的天然血小板激动剂。用[3H]ADP与固定细胞进行的结合研究表明,RPM细胞的结合位点为3.99±1.77×10(5)个/细胞(表观解离常数[kd]=7.75±2.3×10(-8)mol/L),HEL细胞为8.19±3.25×10(5)个/细胞(kd=2.15±0.84×10(-7)mol/L),U937细胞为1.15±0.23×10(6)个/细胞(kd=2.20±0.53×10(-7)mol/L),K562细胞为5.39±2.80×10(5)个/细胞(kd=1.37±0.39×10(-7)mol/L)。用未标记的核苷酸和类似物进行的抑制研究表明,结合具有约85%的特异性,抑制模式与成熟血小板相似。嘌呤碱基腺苷几乎没有抑制作用。这些研究表明,人和大鼠造血细胞系均具有完整的ADP受体,可能是未来研究这个重要血小板激活系统结构和功能的有用工具。

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