Johansen B H, Jensen T, Thorpe C J, Vartdal F, Thorsby E, Sollid L M
Institute of Transplantation Immunology, Rikshospitalet, University of Oslo, N-0027 Oslo, Norway.
Immunogenetics. 1996;45(2):142-50. doi: 10.1007/s002510050182.
We compared the peptide binding specificity of three HLA-DQ molecules; HLA-DQ(alpha1()0501, beta1()0201), HLA-DQ(alpha1()0201, beta1()0202), and HLA-DQ(alpha1()0501, beta1()0301). The first of these molecules confers susceptibility to celiac disease and insulin-dependent diabetes mellitus, while the two latter molecules, which share either the alpha chain or the nearly identical beta chain with HLA-DQ(alpha1()0501, beta1()0201), do not predispose to these disorders. The binding of peptides was detected in biochemical binding assays as inhibition of binding of radiolabeled indicator peptides to affinity-purified HLA-DQ molecules. Binding experiments with several peptides demonstrated a clear difference in peptide binding specificity between the three HLA-DQ molecules. Further, single amino acid substitution analyses indicated that the HLA-DQ molecules have different peptide binding motifs. The experimental data were corroborated by computer modelling analysis. Our data suggest that the three HLA-DQ molecules prefer large hydrophobic residues in P1 of peptides with subtle differences in side-chain preferences. HLA-DQ(alpha1()0501, beta1()0201) and HLA-DQ(alpha1()0201, beta1()0202) both prefer large hydrophobic residues in P9, whereas HLA-DQ(alpha1()0501, beta1()0301) prefers much smaller residues in this position. HLA-DQ(alpha1()0501, beta1()0201) and HLA-DQ(alpha1()0201, beta1()0202), in contrast to HLA-DQ(alpha1()0501, beta1()0301), prefer negatively charged residues in P4 and P7. A less prominent P6 pocket also appears to differ between the three HLA-DQ molecules. Our results indicate that polymorphic residues of both the alpha and the beta chain determine the peptide binding specificity of HLA-DQ(alpha1()0501, beta1()0201), but that the beta chain polymorphisms appears to play the most important role. The information on peptide residues which are advantageous and deleterious for binding to these HLA-DQ molecules may make possible the prediction of characteristic features of peptide that bind to HLA-DQ(alpha1()0501, beta1()0201) and precipitate celiac disease.
我们比较了三种HLA - DQ分子的肽结合特异性;HLA - DQ(α1()0501, β1()0201)、HLA - DQ(α1()0201, β1()0202)和HLA - DQ(α1()0501, β1()0301)。其中第一种分子赋予乳糜泻和胰岛素依赖型糖尿病易感性,而后两种分子,它们与HLA - DQ(α1()0501, β1()0201)共享α链或几乎相同的β链,不会导致这些疾病。在生化结合试验中,通过检测放射性标记的指示肽与亲和纯化的HLA - DQ分子的结合抑制来检测肽的结合。对几种肽的结合实验表明,这三种HLA - DQ分子在肽结合特异性上存在明显差异。此外,单氨基酸取代分析表明,HLA - DQ分子具有不同的肽结合基序。计算机建模分析证实了实验数据。我们的数据表明,这三种HLA - DQ分子在肽的P1位点偏好大的疏水残基,在侧链偏好上有细微差异。HLA - DQ(α1()0501, β1()0201)和HLA - DQ(α1()0201, β1()0202)在P9位点都偏好大的疏水残基,而HLA - DQ(α1()0501, β1()0301)在该位置偏好小得多的残基。与HLA - DQ(α1()0501, β1()0301)相比,HLA - DQ(α1()0501, β1()0201)和HLA - DQ(α1()0201, β1()0202)在P4和P7位点偏好带负电荷的残基。三个HLA - DQ分子之间P6口袋的差异也不太明显。我们的结果表明,α链和β链的多态性残基决定了HLA - DQ(α1()0501, β1()0201)的肽结合特异性,但β链多态性似乎起最重要的作用。关于与这些HLA - DQ分子结合有利和有害的肽残基的信息,可能使预测与HLA - DQ(α1()0501, β1()0201)结合并引发乳糜泻的肽的特征成为可能。
