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自身免疫易感的MRL-lpr/lpr小鼠中不同抗体酶的形成与造血祖细胞集落形成的变化有关。

Formation of different abzymes in autoimmune-prone MRL-lpr/lpr mice is associated with changes in colony formation of haematopoietic progenitors.

作者信息

Andryushkova Alexandra A, Kuznetsova Irina A, Bineva Valentina N, Toporkova Ludmila B, Sakhno Ludmila V, Tikhonova Marina A, Chernykh Elena R, Orlovskaya Irina A, Nevinsky Georgy A

机构信息

Institute of Chemical Biology and Fundamental Medicine, Siberian Branch of the Russian Academy of Sciences, Novosibirsk, Russia.

出版信息

J Cell Mol Med. 2007 May-Jun;11(3):531-51. doi: 10.1111/j.1582-4934.2007.00048.x.

Abstract

It was shown that IgGs from the sera of 2-7-month-old control non-autoimmune (CBA x C57BL)F1 and BALB/c mice and 2-3-month-old autoimmune prone MRL-lpr/lpr mice (conditionally healthy mice) are catalytically inactive. During spontaneous development of deep systemic lupus erythematosus (SLE)-like pathology a specific reorganization of immune system of these mice leads to conditions associated with a production of IgGs hydrolyzing DNA, ATP and polysaccharides with low catalytic activities (conditionally pre-diseased mice).A significant increase in DNase, ATPase and amylase IgG relative activities associated with a transition from pre-diseased to deep diseased mice is correlated with additional changes in differentiation and proliferation of mice bone marrow haematopoietic stem cells (HSCs) and lymphocyte proliferation in different organs. The highest increase in all abzyme activities was found in mice immunized with DNA, which in comparison with pre-diseased and diseased mice are characterized by a different profile of HSC differentiation and by a suppression of cell apoptosis. Abzyme activities in the serum of pregnant females were comparable with those for pre-diseased mice, but the profile of HSC differentiation and cell apoptosis levels in pregnant and pre-diseased mice were quite different. Right after the beginning of lactation (4 days after delivery) and in a late time of lactation (14 days after delivery) there was an observed increase in cell apoptosis and two different stages of significant change in the HSC differentiation profiles; the first stage was accompanied with a significant increase and the second with a remarkable decrease in abzyme activities. Overall, all mouse groups investigated are characterized by a specific relationship between abzyme activities, HSC differentiation profiles, levels of lymphocyte proliferation, and cell apoptosis in different organs. From our point of view, the appearance of ATPase, DNase activities may be considered the earliest statistically significant marker of mouse spontaneous SLE and a further significant increase in their activities correlates with the appearance of SLE visible markers and with an increase in concentrations of anti-DNA Abs and urine protein. However, development of autoimmune (AI)-reactions and the increase in the sera anti-DNA antibodies (Abs) and in the abzyme activities in pregnant and lactating mice do not associate with SLE visible markers and proteinuria. The possible differences in immune system reorganizations during pre-disease, disease, pregnancy and lactation leading to production of different auto-antibodies and abzymes are discussed.

摘要

结果表明,2至7月龄对照非自身免疫性(CBA×C57BL)F1和BALB/c小鼠以及2至3月龄自身免疫易感MRL-lpr/lpr小鼠(条件健康小鼠)血清中的IgG无催化活性。在深度系统性红斑狼疮(SLE)样病理的自然发展过程中,这些小鼠免疫系统的特定重组导致了与产生具有低催化活性的水解DNA、ATP和多糖的IgG相关的状况(条件性疾病前期小鼠)。与从疾病前期小鼠转变为深度患病小鼠相关的DNase、ATPase和淀粉酶IgG相对活性的显著增加,与小鼠骨髓造血干细胞(HSC)的分化和增殖以及不同器官中淋巴细胞增殖的其他变化相关。在用DNA免疫的小鼠中发现所有抗体酶活性增加最为显著,与疾病前期和患病小鼠相比,这些小鼠的HSC分化谱不同且细胞凋亡受到抑制。怀孕雌性小鼠血清中的抗体酶活性与疾病前期小鼠相当,但怀孕小鼠和疾病前期小鼠的HSC分化谱和细胞凋亡水平有很大差异。在哺乳开始后(分娩后4天)和哺乳后期(分娩后14天),观察到细胞凋亡增加以及HSC分化谱发生两个不同阶段的显著变化;第一阶段伴随着抗体酶活性显著增加,第二阶段则显著降低。总体而言,所有研究的小鼠组在抗体酶活性、HSC分化谱、淋巴细胞增殖水平以及不同器官中的细胞凋亡之间存在特定关系。在我们看来,ATPase、DNase活性的出现可能被认为是小鼠自发性SLE最早具有统计学意义的标志物,其活性的进一步显著增加与SLE可见标志物的出现以及抗DNA抗体和尿蛋白浓度的增加相关。然而,怀孕和哺乳小鼠中自身免疫(AI)反应的发展以及血清抗DNA抗体(Abs)和抗体酶活性的增加与SLE可见标志物和蛋白尿无关。本文讨论了在疾病前期、疾病期、怀孕和哺乳期间免疫系统重组可能导致产生不同自身抗体和抗体酶的差异。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fce7/3922359/88d3377d5ef4/jcmm0011-0531-f1.jpg

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