002; Fig. 1b). In addition – and as previously demonstrated [6, 23] – the
pretreatment set-point viral load correlated significantly with the post-STI viral load (P < 0.001). The duration of STI and viral load at pretreatment set point were therefore included in multivariable analyses. Alectinib research buy Eighty-nine patients (68%) carried at least one HLA-B Bw4 allele. Bw4 alleles can be further separated into those carrying isoleucine or threonine at position 80 (Bw4-80Ile and Bw4-80Thr, respectively). Functionally, alleles with isoleucine act as strong ligands, whereas alleles carrying a threonine act as weak ligands of KIR3DL1 [24]. The former were detected in 52 patients (40%) and the latter in 37 patients (28%), whereas 41 patients carried no Bw4 alleles (32%). Patients not carrying a Bw4 allele showed a median post-STI viral load of 3.24 log copies/ml (IQR 2.21–4.29 log copies/ml), whereas the median post-STI viral load was 2.39 log copies/ml (IQR 0–3.62 log copies/ml) in Bw4-positive patients (P = 0.003; Fig. 2a). No difference was found between carriers of 80Thr and 80Ile subgroups of the Bw4 (median increase 2.40 and 2.39 log copies/ml, respectively; P = 0.66; Fig. 2b). We next analysed the impact of allelic diversity within the KIR3DL1 locus in Bw4-positive patients. Of 125 KIR3DL1-positive patients, 84 tested Selleck UK-371804 positive for at least one Bw4
antigen. We found no difference between patients carrying KIR3DL1 alleles with high (*h/*x) and low (*l/*l) surface expression (median increase 2.91 and 2.71 log copies/ml, respectively; P = 0.57; Fig. 2c). Equally, the presence of the KIR3DL1*004 allele DCLK1 – which in conjunction with Bw4 has been shown to delay the progression to AIDS – had no significant impact on post-STI viral loads (median increase 2.65 vs. 2.91 log copies/ml, respectively; P = 0.58; Fig. 2d). The activating receptor KIR3DS1 – which segregates as an allele of KIR3DL1 – was contained in 45 patients’ genotypes (35%), of which 13 also carried Bw4Ile. The presence of KIR3DS1 with Bw4Ile has been shown to delay progression
to AIDS [25]. In our setting, we found no difference in the rise in viral load between KIR3DS1+/Bw4-80Ile+ patients (median increase 2.65 log copies/ml) and patients who did not carry either KIR3DS1 or Bw4-80Ile or both (median increase 2.91 log copies/ml; P = 0.81; Fig. 2e). Finally, we analysed the impact of the SNPs in HCP5 and in HLA-C −35. Nine patients (7%) carried one G allele in the HCP5 locus, and all remaining patients were homozygous for the wild-type T-allele. The median viral load was lower in patients with HCP5-G (median 2.76 log copies/ml) compared with HCP5-TT homozygous patients (median 2.85 log copies/ml). This difference was, however, not statistically significant (P = 0.90; Fig. 2f). At the HLA-C −35 locus, 79 patients (61%) were homozygous for the major T-allele and seven patients (5%) were homozygous carriers of the protective C allele, whereas the remaining 44 patients (34%) carried one copy of each allele.