Association of a 9.2‐kilobase pvu ii class i major histocompatibility complex restriction fragment length polymorphism with ankylosing spondylitis

113

Autoantibodies to phospholipids (APA) occur frequently in systemic lupus erythematosus (SLE) and other autoimmune disorders and predispose to intravascular thromboses. Major histocompatibility complex (MHC) class II alleles (HLA-DR and DQ) were determined by restriction fragment length polymorphisms (RFLP) in 20 patients with APA (lupus anticoagulant). HLA-DQw7 (DQB1 *0301), linked to HLA-DR5 and -DR4 haplotypes, occurred in 70% and was significantly increased compared to 139 race-matched normal controls (P = 0.002, P corrected Ipci = 0.05, odds ratio [OR] = 5.1). Moreover, the frequency of HLA-DQw7 was significantly higher in SLE patients with APA as compared with patients without APA but with other autoantibodies, including anti-Ro and La (P = 0.0001, pc = 0.002, OR = 10.7), anti-Ro alone (P = 0.001, pc = 0.02, OR = 11.2), anti-dsDNA (P = 0.001, pc = 0.02, OR = 7.1), and possibly anti-Sm (P = 0.04, pc = NS, OR = 6.8) and anti-nRNP (U1-RNP) (P = 0.01, pc = NS, OR = 7.8). The DQB1 *0301 allele of DQw7 showed the strongest association, while the frequencies of the DQA1 *0301 (45%) and DQA1 *0501 (50%) alleles did not differ from the controls. Among the HLA-DQB1

Section: Methodsmentioning

confidence: 99%

Molecular analysis of major histocompatibility complex alleles associated with the lupus anticoagulant.

Arnett¹,

Olsen²,

Anderson³

et al. 1991

113

“…"Broad" HLA-DR specificities (DR1, DR2, DR3/6, DR4, DR5(DRwll), DR5(DRwl2), DR7, DRw8, DR9, and DRw1O) were determined either by RFLP analysis of Taq I, Bam HI and Eco RI digested genomic DNA described previously (42) or by polymerase chain reaction (PCR) amplification of 0.5 gg of genomic DNA using the primers DRBAMP-A (5'-CCCCACAGCACGTTTCTTG-3') and DRBAMP-B (5'-CCGCTGCACTGTGAAGCTCT-3'). The PCR was carried out for 30 cycles under the following parameters: denaturation 1 min at 96°C, annealing I min at 55°C, extension 2 min at 72°C.…”

Section: Introductionmentioning

confidence: 99%

Association of amino acid sequences in the HLA-DQB1 first domain with antitopoisomerase I autoantibody response in scleroderma (progressive systemic sclerosis).

Reveille¹,

Durban²,

Clair³

et al. 1992

132

Previous studies in Caucasians with progressive systemic sclerosis (PSS) have suggested associations of antitopoisomerase I (antitopo I) autoantibodies with either serologically defined HLA-DR2 or DR5. To better define class II HLA associations with the antitopo I response, 161 PSS patients (132 Caucasians and 29 American blacks) were studied for antitopo I autoantibodies by immunodiffusion and immunoblotting, and their HLA-DRB1, DRB3, DQA1, and DQB1 alleles were determined by restriction fragment length polymorphic analysis and DNA oligotyping. Among Caucasians with antitopo I, HLA-DR5(DRB1*1101-*1104), DRB3*0202 and DQw3 (DQw7,8,9) were significantly increased in frequency. In American blacks, however, only HLA-DQB1 *0301 (DQw7) was significantly increased. The presence of HLA-DQB1 *0301 (DQw7) and other HLA-DQB1 alleles bearing the uncharged polar amino acid residue tyrosine at position 30 of the outermost domain was found in all antitopo I-positive Caucasian PSS patients compared with 66% of antitopo I-negative PSS patients (pc = 0.007) and 70% of normal controls (pc = 0.008), as well as all antitopo I-positive black patients. The association with HLA-DQB1 was independent of HLA-DR5(DRB1*1101-*1 104) or any other HLA-DRB1, DRB3, or DQA1 alleles. Alternative or additional candidate epitopes for this autoimmune response include alanine at position 38 and threonine at position 77 of these same DQB1 alleles. These data suggest that genetic predisposition to the antitopo I response in PSS is associated most closely with the HLA-DQB1 locus. (J. Clin. Invest. 1992. 90:973-980.)

“…A variety of studies have reported associations of SS with class I MHC specificities, includingHLA-A9 (11,12), B8 (13,14), andB35 (15,16); class II MHC, including HLA-DRl (16)(17)(18)(19), DR3 (14,20) and DR5 (19,(21)(22)(23); and class III MHC, specifically C4 null alleles (15,22). These associations have been generally weak and inconsistent between different centers, and some investigations have even been unable to show any significant HLA associations with SS (24)(25)(26)(27)(28) (33); 10 sg was digested with the restriction endonucleases BamH 1 and TaqI under conditions specified by the manufacturer, and then electrophoresed through an 0.8% agarose gel overnight at 50 V. The gel was then stained in ethidium bromide, photographed, subjected to denaturation and neutralization as described previously (34), and then transferred on to Zetabind membranes. (Cuno, Inc., Meriden, CT).…”

mentioning

confidence: 99%

“…Oligonucleotide probes corresponding to the polymorphisms at positions 25,34,55, and 69 were used forthe hybridizations as supplied by the 11th International Histocompatibility Testing Workshop.…”

mentioning

confidence: 99%

Association of polar amino acids at position 26 of the HLA-DQB1 first domain with the anticentromere autoantibody response in systemic sclerosis (scleroderma).

Reveille¹,

Owerbach²,

Goldstein³

et al. 1992

HLA class II alleles (detected by DNA typing) were determined in 116 Caucasians with systemic sclerosis positive and negative for anticentromere autoantibodies (ACA). Significantly increased frequencies of HLA-DR5(DRw11) (P = 0.009) and the Dw13(DRB1*0403, *0407) subtypes of DR4 (probability corrected, Pc = 0.005) were seen in ACA positive patients, and HLA-DR1 and DRw8 were also increased. These findings appeared to reflect linkage disequilibrium of DR5(DRwll) and many DR4(Dw13) haplotypes with HLADQw7 and DRi with DQw5. In fact, the presence of a DQB1 allele having a polar glycine or tyrosine at position 26 of the DQB1 first domain versus a hydrophobic leucine accounted for 100% of ACA positive Caucasian systemic sclerosis patients compared to 69% ofthe ACA negative SS patients (P = 0.0008) and 71% of Caucasian controls (P = 0.0003) as well as all 7 ACA patients of non-Caucasian background. Furthermore, the genotype frequency of DQB1 alleles lacking leucine at position 26 was 73% in ACA positive SS patients, compared to 42% of ACA negative patients (P = 1.2 X 10-`) and 38% of controls (P = 5.8 X 10-7). These data, then, suggest that the second hypervariable region of the HLA-DQB1 chain may form the candidate epitope associated with the ACA response. (J.