Tang T, Rosenkranz A, Assmann K J, Goodman M J, Gutierrez-Ramos J C, Carroll M C, Cotran R S, Mayadas T N
Department of Pathology, Brigham and Women's Hospital, Boston, Massachusetts 02115, USA.
J Exp Med. 1997 Dec 1;186(11):1853-63. doi: 10.1084/jem.186.11.1853.
Mac-1 (alphambeta2), a leukocyte adhesion receptor, has been shown in vitro to functionally interact with Fcgamma receptors to facilitate immune complex (IC)-stimulated polymorphonuclear neutrophil (PMN) functions. To investigate the relevance of Mac-1-FcgammaR interactions in IC-mediated injury in vivo, we induced a model of Fc-dependent anti-glomerular basement membrane (GBM) nephritis in wild-type and Mac-1-deficient mice by the intravenous injection of anti-GBM antibody. The initial glomerular PMN accumulation was equivalent in Mac-1 null and wild-type mice, but thereafter increased in wild-type and decreased in mutant mice. The absence of Mac-1 interactions with obvious ligands, intercellular adhesion molecule 1 (ICAM-1), and C3 complement, is not responsible for the decrease in neutrophil accumulation in Mac-1- deficient mice since glomerular PMN accumulation in mice deficient in these ligands was comparable to those in wild-type mice. In vitro studies showed that spreading of Mac-1-null PMNs to IC-coated dishes was equivalent to that of wild-type PMNs at 5-12 min but was markedly reduced thereafter, and was associated with an inability of mutant neutrophils to redistribute filamentous actin. This suggests that in vivo, Mac-1 is not required for the initiation of Fc-mediated PMN recruitment but that Mac-1-FcgammaR interactions are required for filamentous actin reorganization leading to sustained PMN adhesion, and this represents the first demonstration of the relevance of Mac-1-FcgammaR interactions in vivo. PMN-dependent proteinuria, maximal in wild-type mice at 8 h, was absent in Mac-1 mutant mice at all time points. Complement C3-deficient mice also had significantly decreased proteinuria compared to wild-type mice. Since Mac-1 on PMNs is the principal ligand for ic3b, an absence of Mac-1 interaction with C3 probably contributed to the abrogation of proteinuria in Mac-1-null mice.
Mac-1(αβ2)是一种白细胞黏附受体,体外实验表明它可与Fcγ受体发生功能相互作用,以促进免疫复合物(IC)刺激的多形核中性粒细胞(PMN)功能。为了研究Mac-1-FcγR相互作用在体内IC介导损伤中的相关性,我们通过静脉注射抗肾小球基底膜(GBM)抗体,在野生型和Mac-1缺陷型小鼠中诱导了一种Fc依赖性抗GBM肾炎模型。最初肾小球PMN的积聚在Mac-1基因敲除小鼠和野生型小鼠中相当,但此后在野生型小鼠中增加,而在突变小鼠中减少。Mac-1与明显配体细胞间黏附分子1(ICAM-1)和C3补体之间缺乏相互作用,并非Mac-1缺陷型小鼠中性粒细胞积聚减少的原因,因为这些配体缺陷型小鼠的肾小球PMN积聚与野生型小鼠相当。体外研究表明,Mac-1基因敲除的PMN在5 - 12分钟时向IC包被培养皿的铺展与野生型PMN相当,但此后明显减少,这与突变中性粒细胞无法重新分布丝状肌动蛋白有关。这表明在体内,Mac-1不是Fc介导的PMN募集启动所必需的,但Mac-1-FcγR相互作用是丝状肌动蛋白重组导致PMN持续黏附所必需的,这首次证明了Mac-1-FcγR相互作用在体内的相关性。PMN依赖性蛋白尿在野生型小鼠中8小时达到峰值,而在Mac-1突变型小鼠的所有时间点均未出现。与野生型小鼠相比,补体C3缺陷型小鼠的蛋白尿也显著减少。由于PMN上的Mac-1是ic3b的主要配体,Mac-1与C3缺乏相互作用可能导致Mac-1基因敲除小鼠蛋白尿消失。
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