人白细胞介素1 α和β信使rna的表达及白细胞介素1在人外周血单核细胞中的活性。

The Journal of molecular and cellular immunology : JMCI Pub Date : 1987-01-01

S Demczuk, C Baumberger, B Mach, J M Dayer

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引用次数: 0

摘要

巨噬细胞来源的淋巴因子白细胞介素1 (IL 1)在调节免疫(细胞和体液)和非免疫反应中起关键作用。例如，不同状态下IL - 1 α和β的相对表达可能对免疫系统对感染的反应成功至关重要。直到最近，IL - 1 mRNA表达和IL - 1生物活性的比较研究还不可能。我们克隆了IL - 1 α和β cdna，并将它们作为探针进行Northern blot分析，以确定有丝分裂原刺激的外周血单个核细胞中其同源mrna的稳态表达与IL - 1活性的关系。通过淋巴细胞活化因子(IL 1/LAF)和单核细胞因子(IL 1/MCF)活性测定IL 1。在凝集素刺激的PBMC中，最大的细胞相关活性在刺激后12和24小时检测到，而最大的细胞外活性出现在24-48小时之间。在相同的培养中，用IL - 1 α和β cDNA探针进行Northern凝胶印迹分析，确定IL - 1 mRNA稳态表达的动力学。在未培养的新鲜分离的PBMC(零时间)中检测不到IL - 1 mrna。这两种IL - 1 mRNA在凝集素刺激后4小时出现，IL - 1 β mRNA在未刺激的培养中也出现。IL - 1 α和β mRNA的稳态水平在48小时内几乎检测不到。在所有时间点，未刺激培养的IL - 1 mRNA水平明显较低。IL - 1 β mRNA总是明显多于IL - 1 α mRNA。较少丰富的IL - 1 α mRNA在IL - 1 β mRNA水平下降之前，其稳态水平下降。在这些培养条件下未检测TNF α活性和mRNA。Poly(A) + RNA注射到爪蟾卵母细胞后，Northern blot检测到IL - 1 mrna具有生物活性。为了了解IL - 1在免疫和非免疫事件中的确切性质，我们认为有必要首先研究IL - 1 mRNA稳态水平与其细胞相关和细胞外生物活性的动力学。本文提供的数据可能有助于更好地理解通过IL - 1表达调节的各种免疫和非免疫反应的病因。

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Expression of human IL 1 alpha and beta messenger RNAs and IL 1 activity in human peripheral blood mononuclear cells.

The macrophage-derived lymphokine interleukin 1 (IL 1) plays a critical role in modulating immune (cellular and humoral) and nonimmune responses. For example, the relative expression of IL 1 alpha and beta under various states may be crucial to the success of the immune system in response to infection. Until recently, a comparative study of IL 1 mRNA expression and IL 1 biological activity was not possible. We have cloned both IL 1 alpha and beta cDNAs and employed them as probes in Northern blot analysis to determine in mitogen-stimulated peripheral blood mononuclear cells the steady-state expression of their cognate mRNAs with respect to IL 1 activity. IL 1 was determined by the lymphocyte-activating factor (IL 1/LAF) and the mononuclear cell factor (IL 1/MCF) activities. In lectin-stimulated PBMC, maximum cell-associated activities whereas detected at 12 and 24 hr after stimulation whereas maximum extracellular activities appeared between 24-48 hr. In the same cultures, the kinetics of IL 1 mRNA steady-state expression were determined by Northern gel blot analysis with IL 1 alpha and beta cDNA probes. IL 1 mRNAs were undetectable in noncultured freshly isolated PBMC (time zero). Both IL 1 mRNAs appeared as early as 4 hr after lectin stimulation as did IL 1 beta mRNA in unstimulated cultures. Both IL 1 alpha and beta mRNA steady-state levels were barely detectable by 48 hr. At all time points, IL 1 mRNA levels were considerably lower in unstimulated cultures. IL 1 beta mRNA was always considerably more abundant than IL 1 alpha mRNA. The less abundant IL 1 alpha mRNA showed a decrease in its stead-state levels prior to the reduction in the levels of IL 1 beta mRNA. TNF alpha activity and mRNA were not detected under these culture conditions. Poly(A) + RNA injected into Xenopus oocytes revealed that the Northern blot detected IL 1 mRNAs were biologically active. To understand the precise nature of IL 1 in immune and nonimmune events, we felt it necessary to first study the kinetics of IL 1 mRNA steady-state levels with respect to its cell-associated and extracellular biological activities. The data presented here may allow for a better understanding of the etiology of various immune and nonimmune responses that are modulated through the expression of IL 1.

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The Journal of molecular and cellular immunology : JMCI

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