HLA,唾液IgA和变形链球菌——有关系吗?

Swedish dental journal. Supplement Pub Date : 2004-01-01
Marie Louise Lundin Wallengren
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引用次数: 0

摘要

本研究的目的是探讨人白细胞抗原(HLA)复合物、变形链球菌定植和唾液免疫球蛋白a (IgA)抗体对抗变形链球菌抗原之间的可能关系。在第一项研究中,在一组肾移植患者(I)中观察到HLA- dr4与变形链球菌水平之间存在强烈的负相关关系。在一组健康献血者中观察到类似的趋势(I)。在第二项研究(II)中,也观察到这种趋势。由于HLA分子调节唾液中抗体的产生,在接下来的研究(III)中,研究了hla - dr4阳性和dr4阴性人群唾液中对三种口腔链球菌的IgA活性。研究发现,与hla - dr4阴性人群相比,hla - dr4阳性人群,尤其是DRB1*0401和DRB1*0404亚组的IgA活性较弱,尤其是对变形链球菌的IgA活性较弱。然而,免疫印迹所揭示的免疫反应模式往往是复杂的,对于更大的研究人群的进一步研究,揭示检测到的抗原的性质至关重要。在第四项研究(IV)中,用Western blot方法分析了未经处理的唾液以及细胞表面反应性IgA被整个细菌细胞吸收的唾液对不同口腔链球菌的影响。吸收后缺失的高分子带可能代表细胞表面抗原,因此它们可能参与粘附机制并可在体内阻断。在接下来的研究(V)中,我们在更大的人群中研究了唾液对三种口腔链球菌细胞表面抗原的IgA活性与不同HLA-DRB1*4等位基因的关系。结果显示,与其他DRB1*04型相比,DRB1*0401和*0404亚群对变形链球菌、sobrinus和链球菌抗原(SA) I/II的免疫印迹条带较少,强度也较低,而副anguis则没有。本论文的主要结论是,个体的HLA谱似乎会影响唾液对变异链球菌抗原的IgA反应,从而也可能影响口腔中细菌的状况。
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HLA, salivary IgA and mutans streptococci--is there a relation?

The aim of the present studies was to investigate a possible relationship between the human leukocyte antigen (HLA) complex, colonization of mutans streptococci and salivary immunoglobulin A (IgA) antibodies against mutans streptococcal antigens. In the first study a strong inverse relationship between HLA-DR4 and levels of mutans streptococci was observed for a group of renal transplant patients (I). In a group with healthy blood-donors a similar trend was observed (I). This tendency was also seen for a selected population investigated in the second study (II). Since the HLA molecules regulate the production of antibodies in saliva, the salivary IgA activity to three oral streptococci in a population of HLA-DR4-positive and DR4-negative subjects was investigated in the following study (III). It was found that the HLA-DR4-positive subjects, especially the DRB1*0401 and DRB1*0404 subgroups, showed a weaker IgA activity, in particular to Streptococcus mutans, as compared to the HLA-DR4-negative. However, immune response patterns revealed by Western blotting are often complex and for further studies with larger study populations it was crucial to unravel the nature of the detected antigens. In the fourth study (IV), untreated saliva, as well as saliva, in which cell-surface reactive IgA had been absorbed with whole bacteria cells, were analysed in Western blot against different oral streptococci. The high molecular bands, that were absent after absorption, likely represented cell-surface antigens and were thus of interest as they might be involved in adhesion mechanisms and available for blocking in vivo. In the next study (V), the salivary IgA activity to cell-surface antigens of three oral streptococci in relation to different HLA-DRB1*4 alleles was studied in a larger population. The immunoblots were analysed in a computer program and intensity graphs revealed that the DRB1*0401 and *0404 subgroups, compared to other DRB1*04 types, showed fewer as well as less intense immunoblot bands to antigens from S. mutans, S. sobrinus and streptococcal antigen (SA) I/II, but not S. parasanguis. The main conclusion from this thesis is that the HLA profile of the individual seems to influence the salivary IgA response to mutans streptococcal antigens and might thus also affect the conditions for the bacteria in the oral cavity.

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