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Synergistic signals in the mechanism of antigen-induced exocytosis in 2H3 cells: evidence for an unidentified signal required for histamine release

机译:2H3细胞中抗原诱导的胞吐作用机理中的协同信号:组胺释放所需信号尚不明确的证据

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摘要

The aim of this study was to determine whether the increase in cytosolic free Ca2+ concentration ([Ca2+]i) in response to antigen (aggregated ovalbumin) on IgE-primed 2H3 cells was sufficient to account for exocytosis. When the [Ca2+]i responses to antigen and the Ca2+ ionophore A23187 were compared, A23187 was much less effective at releasing histamine at equivalent [Ca2+]i increases, and little or no stimulated histamine release occurred with A23187 concentrations that matched the [Ca2+]i response to antigen concentrations that stimulated maximal histamine release. The [Ca2+]i response to antigen is not, therefore, sufficient to account for exocytosis, although extracellular Ca2+ is necessary to initiate both the [Ca2+]i response and histamine release: the antigen must generate an additional, unidentified, signal that is required for exocytosis. To determine whether this signal was the activation of protein kinase C, the effects of the phorbol ester 12- 0-tetradecanoyl phorbol 13-acetate (TPA) on the responses to antigen were examined. TPA blocked the antigen-induced [Ca2+]i response and the release of inositol phosphates but had little effect on histamine release and did not stimulate exocytosis by itself. The unidentified signal from the antigen is therefore distinct from the activation of protein kinase C and is generated independently of the [Ca2+]i response or the release of inositol phosphates. Taken together with other data that imply that there is very little activation of protein kinase C by antigen when the rate of histamine release is maximal, it is concluded that the normal exocytotic response to antigen requires the synergistic action of the [Ca2+]i signal together with an unidentified signal that is not mediated by protein kinase C.
机译:这项研究的目的是确定在IgE启动的2H3细胞上对抗原(聚集的卵清蛋白)的反应中游离的Ca2 +浓度([Ca2 +] i)的增加是否足以说明胞吐作用。当比较对抗原的[Ca2 +] i反应和Ca2 +离子载体A23187时,A23187在等效[Ca2 +] i增加时释放组胺的效果要差得多,并且与[Ca2 +]匹配的A23187浓度几乎没有或没有刺激组胺的释放。我对刺激最大组胺释放的抗原浓度有反应。因此,对抗原的[Ca2 +] i反应不足以说明胞吐作用,尽管细胞外Ca2 +对于启动[Ca2 +] i反应和组胺释放都是必需的:抗原必须产生所需的其他未鉴定信号用于胞吐作用。为了确定该信号是否是蛋白激酶C的活化,检查了佛波酯12-0-十四烷酰基佛波13-乙酸酯(TPA)对抗原应答的作用。 TPA阻断了抗原诱导的[Ca2 +] i反应和肌醇磷酸酯的释放,但对组胺的释放几乎没有影响,并且本身不刺激胞吐作用。因此,来自抗原的未知信号不同于蛋白激酶C的激活,并且独立于[Ca2 +] i反应或肌醇磷酸酯的释放而产生。结合其他数据表明当组胺释放速率最大时抗原对蛋白激酶C的激活非常少,可以得出结论,对抗原的正常胞吐反应需要[Ca2 +] i信号共同发挥协同作用。其信号不是由蛋白激酶C介导的。

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  • 年度 1987
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