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携带lpr基因的MRL/Mp和C57BL/6J小鼠中白细胞介素2活性不足。

Deficient interleukin 2 activity in MRL/Mp and C57BL/6J mice bearing the lpr gene.

作者信息

Wofsy D, Murphy E D, Roths J B, Dauphinée M J, Kipper S B, Talal N

出版信息

J Exp Med. 1981 Nov 1;154(5):1671-80. doi: 10.1084/jem.154.5.1671.

Abstract

Spleen cells from MRL-lpr and B6-lpr mice have a marked defect in the ability to produce interleukin 2 (IL-2) in response to concanavalin A stimulation. This defect precedes the onset of clinical illness, increases with age, and eventually becomes virtually absolute. It is not due to cellular suppression of IL-2 production, nor does it reflect the presence of a soluble inhibitor of IL-2 activity. Failure to restore IL-2 production with macrophage-replacing factors, such as interleukin 1 and phorbol myristic acetate, suggests that IL-2 deficiency reflects a primary T cell defect rather than a macrophage defect. MRL-lpr and B6-lpr spleen cells also have an age-dependent reduction in IL-2 response that apparently results from a deficiency of cell surface receptors for IL-2. Congenic MRL-+/+ and B6-+/+ mice, which lack the lpr gene responsible for accelerated autoimmunity and lymphoproliferation, have normal IL-2 activity. These findings suggest that a defect in IL-2 activity may contribute to impaired immunoregulation in mice bearing the lpr gene. The absence of such a defect in MRL-+/+ and B6-+/+ mice further suggests that a single autosomal recessive gene is responsible for IL-2 deficiency.

摘要

来自MRL - lpr和B6 - lpr小鼠的脾细胞在对刀豆球蛋白A刺激产生白细胞介素2(IL - 2)的能力方面存在明显缺陷。这种缺陷在临床疾病发作之前就已出现,随年龄增长而加重,最终几乎完全丧失。它不是由于细胞对IL - 2产生的抑制作用,也不反映存在IL - 2活性的可溶性抑制剂。用巨噬细胞替代因子(如白细胞介素1和佛波酯)无法恢复IL - 2的产生,这表明IL - 2缺乏反映的是原发性T细胞缺陷而非巨噬细胞缺陷。MRL - lpr和B6 - lpr脾细胞对IL - 2的反应也随年龄增长而降低,这显然是由于IL - 2细胞表面受体缺乏所致。缺乏导致自身免疫加速和淋巴细胞增殖的lpr基因的同基因MRL - +/+和B6 - +/+小鼠具有正常的IL - 2活性。这些发现表明,IL - 2活性缺陷可能导致携带lpr基因小鼠的免疫调节受损。MRL - +/+和B6 - +/+小鼠不存在这种缺陷,这进一步表明单个常染色体隐性基因是导致IL - 2缺乏的原因。

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