Progressive increase in central nervous system immune activation in untreated primary HIV-1 infection

ART-naïve HIV-1-infected subjects within one year of transmission were recruited in Gothenburg, Sweden (n = 17) and San Francisco, United States (n = 64). As described previously [16], PHI in the participants was confirmed by a combination of seroconversion, nucleic acid testing, or less-sensitive enzyme-linked immunosorbent assay (ELISA) testing, according to the serologic testing algorithm for recent HIV seroconversion (STARHS) methods [17]. The duration since transmission was estimated by considering the date at onset of seroconversion symptoms as 14 days post-transmission [18]. For participants without seroconversion symptoms (n = 16), we estimated the date of transmission as halfway between the most recent negative and positive HIV tests [19]. Protocols were approved by the University of California San Francisco Committee on Human Research (H9133-26278) and the Research Ethics Committee of the University of Gothenburg (Ö588-01). Informed consent was obtained from all participants prior to enrollment.

Longitudinal paired samples of CSF and blood were obtained prior to cART. In San Francisco, visits were scheduled at baseline (earliest enrollment after initial transmission), six weeks, and every subsequent six months from baseline, while in Gothenburg, study intervals were variable. Opportunistic infections and major neurological diseases such as stroke, multiple sclerosis, and seizure disorders were ruled out at baseline. Blood samples were analyzed for HIV RNA, albumin, CD4+ lymphocytes and CD8+ lymphocytes, and CSF samples were analyzed for HIV RNA, albumin, and white blood cell (WBC) count, as previously described [16]. Concentrations of CSF and blood neopterin were measured in previously frozen samples in the laboratory of Dr Fuchs by commercial immunoassays (BRAHMS Aktiengesellschaft, Hennigsdorf, Germany). A subset of fresh whole blood and CSF samples obtained in San Francisco (n = 42) was further analyzed by multiparameter flow cytometry as previously described [20],[21] using FACSDiva (BD Biosciences, San Jose, USA) to measure the percentage of CD4+ and CD8+ cells with dual positivity for activation markers CD38 and HLA-DR. Data was analyzed with FlowJo (TreeStar, Ashland, Oregon, United States).

All statistical analyses were performed using SPSS version 19, IBM Corp., Armonk, USA. All descriptive statistics are presented as median and interquartile range (IQR) for continuous variables, and as frequency (%) for categorical variables. Fischer’s exact test, the Mann-Whitney U test, and Spearman’s rank correlation coefficient were used where appropriate.

This model yielded a regression coefficient for slope (change in CSF neopterin per day post-transmission) equal to 0.000294 - 1.397E-5 × baseline CSF neopterin, suggesting that the slope of CSF neopterin trajectory was dependent on baseline CSF neopterin. Based on this regression coefficient, baseline CSF neopterin values greater than 21 nmol/L yielded a negative slope, whereas baseline CSF neopterin values less than 21 nmol/L yielded a positive slope. Therefore, a baseline CSF neopterin level of 21 nmol/L was a cutoff value that determined the increasing versus decreasing trajectory of CSF neopterin. These results were confirmed by another model that used baseline CSF neopterin as a dichotomous variable (above or below 21 nmol/L). Although only the group with baseline CSF neopterin below 21 nmol/L included subjects with visits beyond 150 weeks, sensitivity analysis constraining the time axis to 150 weeks yielded the same trajectories as above. Therefore the full analysis, which included these visits, is presented in this paper.

Similarly, we used mixed-effects models to examine trends in the proportions of CD4+ and CD8+ cells co-expressing CD38 and HLA-DR in blood and CSF. In each of the four models, days post-transmission was a fixed effect, intercept was a random effect, and the percentage of cells co-expressing CD38 and HLA-DR was the outcome variable.

The characteristics of participants are shown in Table 1. Subjects were mostly male, had a median age of 36 years (IQR: 28 to 45), and were at a median of 100 days post-transmission at baseline. Although the median blood CD4+ T-cell count was 552 cells/μL (IQR: 389 to 720), one individual had an extremely low baseline CD4+ T-cell count of 111 cells/μL. The total number of visits ranged from 1 to 13, and the median duration of follow-up was 321 days.

Consistent with a previous report on a subset of this cohort [16], the median CSF neopterin concentration at baseline was 10.2 nmol/L (IQR: 6.6 to 21.3), with 81% of subjects having levels above 5.8 nmol/L, the upper limit of normal (ULN) [22]. Plasma neopterin at baseline was also elevated at 15.1 nmol/L (IQR: 9.4 to 21.6, ULN: 8.7 nmol/L [23]). Percentages of activated CD4+ and CD8+ cells in both blood and CSF were also elevated compared to published values in HIV-uninfected subjects obtained using similar methods (Table 1) [20]. Plasma neopterin correlated positively with the percentage of activated CD4+ cells (r_s = 0.38, P = 0.02) and CD8+ cells (r_s = 0.40, P = 0.02) in blood, and the percentage of activated CD8+ cells in CSF (r_s = 0.41, P = 0.01). CSF neopterin correlated moderately with the percentage of activated CD4+ cells (r_s = 0.36, P = 0.03) and CD8+ cells (r_s = 0.37, P = 0.03) in blood and strongly correlated with the percentage of activated CD8+ cells in CSF (r_s = 0.63, P <0.001).

To confirm the observation of 21 nmol/L as a cutoff value, we ran a similar mixed-effects model with baseline CSF neopterin as a categorical variable. This model yielded the average change in CSF neopterin level over time separately for the low and high groups, and showed that they were significantly different as evidenced by the group-by-time interaction (P <0.001). As shown in Figure 1, CSF neopterin concentration increased in the low group by approximately 2.9% per 10 weeks (P <0.001), and decreased in the smaller high group by approximately 6.7% per 10 weeks (P = 0.001).

When the groups with baseline CSF neopterin concentrations below and above 21 nmol/L were compared on baseline parameters (Table 2), significant differences were not found in age or days post-transmission. However, the high group was found to have a lower CD4+ cell count in blood (P <0.001), higher neopterin levels in plasma (P = 0.006) and CSF (P <0.001), and HIV RNA levels in both plasma (P = 0.02) and CSF (P = 0.006) that were greater by more than an order of magnitude. In both groups, the level of HIV RNA in CSF was lower than that found in plasma.

Despite a higher CSF-to-plasma neopterin ratio in the high group (Figure 2A, P <0.001), the two groups did not differ in the CSF-to-plasma HIV RNA ratio (Figure 2B, P = 0.37) or the CSF-to-plasma albumin ratio (Figure 2C, P = 0.06). The neopterin-to-HIV RNA ratio was higher in the high group in CSF (P <0.001) but not in plasma (P = 0.10).

Clinically, two out of 33 subjects in the low group (5.9%) and one out of 11 subjects in the high group (9.1%) had specific neurological seroconversion symptoms (excluding headache). The two neurosymptomatic patients in the low group had Guillain-Barré-like syndrome and meningitis, and the one patient in the high group had meningitis.

Mixed-model analyses of subjects with available flow cytometry data (n = 42) showed an increasing trend in the percentage of activated CD4+ cells in blood at a rate of 0.23 per 10 weeks (P = 0.05, Figure 3A). A significant trend for activated CD8+ cells in blood was not found (P = 0.54, Figure 3B). In CSF, the percentage of activated CD4+ cells increased at a rate of 0.63 per 10 weeks (P = 0.04). We noted an outlier value that had a sharp increase from 8 to 54% from day 26 to 51 post-transmission; re-analysis excluding this outlier yielded a rate of 0.8 per 10 weeks (P <0.001, Figure 3C). The percentage of activated CD8+ cells in CSF increased at a rate of 0.73 per 10 weeks (P = 0.02, Figure 3D).