Abstract
Understanding the determinants of broadly neutralizing antibody (bNAb) evolution is crucial for the development of bNAb-based HIV vaccines1. Despite emerging information on cofactors that promote bNAb evolution in natural HIV-1 infections, in which the induction of bNAbs is genuinely rare2, information on the impact of the infecting virus strain on determining the breadth and specificity of the antibody responses to HIV-1 is lacking. Here we analyse the influence of viral antigens in shaping antibody responses in humans. We call the ability of a virus strain to induce similar antibody responses across different hosts its antibody-imprinting capacity, which from an evolutionary biology perspective corresponds to the viral heritability of the antibody responses. Analysis of 53 measured parameters of HIV-1-binding and neutralizing antibody responses in a cohort of 303 HIV-1 transmission pairs (individuals who harboured highly related HIV-1 strains and were putative direct transmission partners or members of an HIV-1 transmission chain) revealed that the effect of the infecting virus on the outcome of the bNAb response is moderate in magnitude but highly significant. We introduce the concept of bNAb-imprinting viruses and provide evidence for the existence of such viruses in a systematic screening of our cohort. The bNAb-imprinting capacity can be substantial, as indicated by a transmission pair with highly similar HIV-1 antibody responses and strong bNAb activity. Identification of viruses that have bNAb-imprinting capacities and their characterization may thus provide the potential to develop lead immunogens.
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Main
The capacity to evoke highly similar bNAb responses across vaccinees is crucial for an effective HIV-1 immunogen. Closely related HIV-1 strains may induce similar neutralization responses, as observations from mother-to-child transmission suggest3. To formally evaluate the virus-dictated heritability of antibody responses, we investigated the imprinting capacity of HIV-1 antibody responses within transmission pairs. We designed our study to address two central problems (Extended Data Fig. 1a, b). First, we investigated whether the same virus, when transmitted to two different people, induces similar binding and neutralizing antibody responses (imprints a similar antibody response). Second, we investigated how promising HIV-1 strains with superior bNAb-imprinting capacity can be identified.
On the basis of the Swiss 4.5K Screen4,5, we established a large, adult transmission-pair cohort (n = 303 putative transmission pairs) with comprehensive information on HIV-1-binding and neutralizing antibody responses (Extended Data Fig. 1a). Extensive data on HIV-binding antibody reactivity encompassing IgG1, IgG2 and IgG3 reactivity with 13 antigens was available for all 606 patients from previous analyses5 (Supplementary Data 1). Neutralization activity was assessed against a 14 multi-clade virus panel (Extended Data Fig. 2a and Supplementary Data 1, 2) and evaluated by breadth and a cumulative neutralization score, reflecting potency and breadth across the analysed virus panel (Extended Data Fig. 2a–d). Overall, the neutralization activity in the transmission pair cohort showed the typical pattern seen in chronic infection4: the majority of patients displayed no or low neutralization activity (73% of patients had below 10% breadth).
We hypothesized that if virus-associated factors are important in determining antibody responses, HIV antibody response patterns should be similar in transmission pairs. Using the established 53 HIV-1 antibody parameters (14 neutralization and 39 binding antibody parameters), we conducted a systematic assessment of the HIV-1 antibody imprinting capacity in transmission pairs (Extended Data Fig. 2e).
We detected a significant, positive association of the transmitter and recipient neutralization responses to 7 of the 14 panel viruses (Fig. 1a and Extended Data Fig. 3a). The overall similarity of the neutralization fingerprint within pairs across the 14 panel viruses was assessed as average Spearman correlation (ρSpearman-average) of their neutralization activity (Fig. 1b). To determine the statistical significance of the observed similarity, we used shuffling approaches that randomly reassign recipients to transmitters, thus generating a distribution for the null-expectation of no association. Neutralization fingerprints in observed transmission pairs proved on average positively and significantly associated (ρSpearman-average = 0.11, Pshuffling < 0.001; Fig. 1b). To confirm the influence of the infecting virus, we estimated the heritability of antibody responses by two alternative methods adjusting for the influence of various host, viral and disease factors that are known to influence antibody responses4,5. First, we restricted the shuffling to pairs with the same infection length, subtype and ethnicity (Fig. 1b). Second, we considered mixed-effect Tobit models adjusted for key drivers of HIV-1 antibody development (infection length, ethnicity, virus load and viral diversity) and bNAb specificity (HIV-1 pol subtype) (Fig. 1c). Both approaches confirmed a significant, within-pair correlation of neutralization (Fig. 1b, c). Although other, not yet defined, non-virus-associated factors common to both transmission partners may exist, our data strongly suggest that the infecting virus strain affects the development of neutralization responses. The effects (Fig. 1a, b) remained robust when restricting the analysis to pairs infected with subtype B virus, indicating that the effect is not driven by specific subtypes (Extended Data Fig. 4a, b).
Unravelling the quantitative contribution of the infecting virus to the neutralization response is of particular importance for vaccine development. The mixed-effect Tobit models revealed that, on average, 13.2% of the variability of the neutralization response can be explained by the infecting virus (Fig. 1c). Notably, various alternative models adjusted for cofactors of HIV-1 antibody induction—such as viral load or duration of infection—yielded similar results (9.3–13.8% neutralization variability explained by the virus; Extended Data Fig. 3b). Comparable results were also obtained when we restricted the analysis to the 184 pairs in which both individuals were infected for three or more years (neutralization heritability in Tobit models: 13.2% unadjusted, 9.3% fully adjusted) or when we used multiple imputation instead of a complete case analysis in the fully adjusted model (10.9% neutralization variability; Extended Data Fig. 3c).
HIV-1 antigen-binding activities were also significantly correlated within transmission pairs, but the degree of correlation differed considerably across antigens and IgG classes (Fig. 1a). IgG1 reactivity, the most prominent IgG response in HIV-1 infection5, displayed the highest similarity in transmission pairs (Fig. 1a, b), followed by IgG3 and IgG2 responses. Of note, IgG2 responses, which are only present at low levels during HIV-1 infection, showed no statistically significant similarity at the level of individual antigens. The average within-pair similarity across antigens was nevertheless significantly positive for all three IgG subclasses, with and without taking potentially confounding parameters into account (Fig. 1b). As observed for neutralization responses, the findings remained significant when the analysis was restricted to subtype B infection (Extended Data Fig. 4c, d). The effect of the infecting virus was comparable in magnitude to the effect on neutralization (19%, 7% and 10% for IgG1, IG2 and IgG3 responses, respectively), with similar values observed after adjustment for analysed cofactors of HIV-1 antibody induction (Fig. 1c). The identified influence of the infecting virus on the heritability of HIV-1 binding and neutralizing antibody responses was robust, as confirmed by additional sensitivity analyses (Extended Data Figs. 3b, 5a–c).
The overall effect sizes of the influence of virus genetics on neutralizing and binding antibodies that we report here must be considered as lower bound estimates, as neutralization breadth is generally low in HIV-1 infection. Furthermore, as our cohort setup did not allow assessing matched time points, transmission partners had experienced different lengths of virus replication and antibody response development at sample collection. Although the effects that we identified across the cohort were moderate, individual cases may substantially exceed the observed average antibody similarity. In support of this, two HIV-1 subtype B-infected elite neutralizers (top 1% of neutralizers identified in the Swiss 4.5K Screen4) formed one transmission pair (0.0058 HIV-1 pol genetic distance) that stood out in both potency and breadth (Fig. 2a, b). This pair was subsequently verified by their shared treating physician as a mixed ethnicity heterosexual couple in a stable partnership (T282 female (North African) to R282 male (Asian) transmission). Identification of transmission pairs and genetic subtype information in our cohort is based on pol sequence data collected early after diagnosis. We performed full-genome next-generation sequencing of plasma viruses from T282 and R282 at the time point analysed for antibody reactivity to rule out later superinfection. The obtained consensus full-genome sequences confirmed closely related subtype B viruses in T282 and R282 (Extended Data Fig. 6a). Because the analysed samples of T282 and R282 were collected 1.9 and 3.4 years after the putative transmission event, respectively, considerable genetic differences in Env between the pair were expected6. Env similarity in the pair was nevertheless evident, as highlighted by phylogenetic comparison, validating the close relatedness of the viruses infecting the transmission partners (Fig. 2c). The same pattern was observed for two other transmission pairs (T11–R11 and T294–R294) analysed for comparison.
In line with reactivity to an originally highly related Env antigen, neutralization fingerprint analysis of plasma samples from T282 and R282 in a 42-virus panel confirmed highly similar neutralization responses in this pair (ρSpearman = 0.576; Fig. 2d). Delineation of plasma bNAb specificity by fingerprint analyses (Fig. 2e and Supplementary Data 2) and mutant-virus neutralization mapping (Extended Data Fig. 7a) showed that both partners developed a CD4 binding-site-directed bNAb plasma response and that additional V3 glycan bNAb activity was present in the transmitter.
The occurrence of a transmission pair with such pronounced neutralization strength and similarity in neutralization responses is unlikely to be by chance. By randomly reassigning recipients to transmitters (106 replicates), we determined that the probability of such a strong shared neutralization strength by chance is Pshuffle = 0.017 (Fig. 2a). Although additional non-virus-linked factors that positively influence similar bNAb development may exist, our results point to a considerable influence of the transmitted virus in this elite bNAb-inducing pair. This strongly suggests the existence of virus envelopes with strong bNAb-imprinting capacity that will need to be identified for use in vaccine development.
We next developed a systematic, statistical approach (Extended Data Fig. 8) to identify pairs in which both partners developed notable neutralization strength (assessed by the lower neutralization score reached by one partner) and had similar neutralization and binding responses (Fig. 3a). Using various thresholds for the neutralization strength (n = 7) and the within-pair similarity index (n = 4) of the antibody response, we identified for each combination of thresholds the bNAb-imprinting capacity in our cohort. We counted the number of transmission pairs with a certain neutralization strength and a certain similarity index (exemplified for thresholds of neutralization = 5 and similarity = 0.5 in Fig. 3a, b). For all tested threshold criteria, we identified substantially more candidate transmission pairs with bNAb-imprinting capacity than would be expected by chance (Fig. 3c, d). This indicates that the transmitted HIV-1 strains in these pairs are promising candidates for imprinting highly similar neutralization responses.
Even though the viral Env antigen must certainly have a role, it is conceivable that bNAb-imprinting capacity might also, in part, depend on other virus traits, or demographic, host genomic, or transmission route-related factors. We therefore investigated the influence of known factors implicated in HIV-1 antibody development on bNAb-imprinting capacity in our cohort (Extended Data Fig. 7b, c). BNAb-imprinting capacity was detected more frequently among transmission pairs in which both partners had been infected for three or more years before assessment of antibody reactivity (Extended Data Fig. 7c). This is in line with the generally higher frequency of bNAb induction after prolonged exposure to HIV-14. None of the other tested factors was significantly associated with bNAb-imprinting capacity (Extended Data Fig. 7b, c). Owing to the cross-sectional study set-up, we lacked the means to compare antibody responses at matched time points of infection and, therefore, our findings probably represent an underestimation of the frequency of bNAb-imprinters. Although our transmission cohort is one of the largest described to date, it may still require substantially larger cohorts and specifically tailored studies to detect more subtle influences of cofactors on bNAb imprinting.
The formal assessment of virus-induced heritability of the antibody response performed here quantifies the impact of HIV-1 immunogens on inducing qualitatively and quantitatively similar neutralizing and binding antibody responses. The effect of the infecting virus we observed across the assessed large, cross-sectional, natural history cohort of HIV-1 transmission pairs was significant, ranging between 7 and 19% depending on the antibody response considered (Fig. 1c). This is lower in magnitude than the effect of virus genetics on HIV-1 set point viral load (29%)7,8 but comparable to the effect of virus genetics on CD4+ T cell decline (17%)7,8 and the effect of host genetics of HLA and CCR5 SNPs (14.5%)9. Notably, owing to the cross-sectional nature of the transmission cohort, sampling time points of pairs were not matched for duration of infection. Adjustment for infection time controlled for this in the estimate of the overall imprinting capacity (Fig. 1c). Although in patients with shorter infection times, bnAb-imprinting capacity may have been missed (Fig. 3), the fact that we observe a significant genetic effect of the virus in a cross-sectional, natural history cohort is a clear indication of the strength of our results.
Using a statistical approach to systematically screen for virus strains with bnAb-imprinting capacity, we show that only a minority of HIV-1 transmissions exhibit transferability of strong neutralization antibody traits, suggesting that only some virus strains or Env variants harbour bnAb-imprinting capacity. bnAb-imprinting capacity may be a genuine feature of certain Env variants or a temporal issue, as epitopes needed to evoke a specific neutralization response may be presented only transiently until escape mutations establish. Depending on when, with respect to viral evolution in the transmitter, the transmission occurred, the recipient may not have been exposed to the relevant epitope. If virus escape limits the heritability of antibody responses, transmission during acute HIV-1 infection (where neutralization activity is still low and hence neutralization escape is scarce) should show a higher similarity of antibody responses in transmitter and recipients. However, we found no evidence for higher frequencies of bnAb-imprinting capacity amongst acute phase transmission cases in our cohort (Extended Data Fig. 7c), suggesting that virus escape is not the main limiting factor and that higher patient numbers would be needed to uncover more subtle effects. In general, the fact that bnAb-imprinting upon transmission occurs strongly suggests that relevant epitopes that allow germline triggering can be preserved over longer time periods, for instance as a result of partial escape that retains bnAb-binding capacity10,11.
Although the average effect of virus genetics across the entire cohort was moderate, individual cases with high antibody similarity and capacity to imprint a bNAb immune response can exist. The elite-neutralizing transmission pair that we identified highlights that distinct strains may exist, which harbour the potential to evoke highly similar bNAb and binding antibody responses across individuals. Further studies that identify more such pairs and a detailed characterization of the transmitted strains, longitudinal envelope evolution and the evoked bNAb responses will be needed to understand which specific features render a strain a bNAb imprinter. Clearly, if bNAb-imprinting strains exist, they need to be specifically investigated and characterized. In particular, envelope proteins from bNAb imprinters with proven in vivo transferability of antibody reactivity may provide the ultimate candidate immunogen(s) on which to base bNAb vaccine design.
Methods
Data reporting
No statistical methods were used to predetermine sample size. The experiments were not randomized. The investigators were blinded to allocation (transmitter–recipient pairing) during initial antibody response analyses (all binding antibody responses and neutralization analyses to an eight-virus multi-clade panel. The investigators were not blinded during outcome assessment and extended neutralization analyses.
Study populations and ethics information
The starting cohort for our analysis were 4,281 chronic HIV-1-infected individuals included in a population-wide screen for HIV-1 neutralization breadth, now termed the Swiss 4.5K Screen4, for which extensive plasma neutralization and HIV-1 binding data were generated in a separate study5 (Extended Data Fig. 1a). Detailed information on the plasma sample/patient selection and study design of the Swiss 4.5K Screen has been previously described4 (Extended Data Fig. 1a). All plasma samples were collected during viraemic periods (no antiretroviral treatment at sampling time point) from adult, chronically infected HIV-1 patients. Because the cross-sectional sample selection was pre-determined by the Swiss 4.5K Screen, it was not possible during our current study to select samples matched for infection length or for closeness to putative transmission time points. Important for the interpretation of specific findings in the current study, the study design of the Swiss 4.5K Screen included three patient groups that differed in infection length (1–3, 3–5 and ≥5 years of untreated HIV-1 infection). The highest frequency of neutralization breadth was observed among individuals infected for >3 years4. The plasma samples analysed previously4,5 and in the current study were provided by the biobanks of the Swiss HIV Cohort study (SHCS) and the Zurich Primary HIV Infection Study (ZPHI).
The SHCS and the ZPHI have been approved by the ethics committee of the participating institutions (Kantonale Ethikkommission Bern, Ethikkommission des Kantons St. Gallen, Comite departemental d’ethique des specialites medicales et de medicine communataire et de premier recours, Hôpitaux Cantonale de Genève, Kantonale Ethikkommission Zürich, Repubblica e Cantone Ticino—Comitato Ethico Cantonale, Commission cantonale d'étique de la recherche sur l'être humain, Canton de Vaud, Lausanne, Ethikkommission beider Basel for the SHCS and Kantonale Ethikkommission Zürich for the ZPHI) and written informed consent had been obtained from all participants. Please see the supplementary note of the previous study4 and the Supplementary Methods of the current study for further details on the cohorts and the collected patient data. The SHCS is a prospective, nationwide, longitudinal, non-interventional, observational, clinic-based cohort with semi-annual visits and blood collections, enrolling all HIV-infected adults living in Switzerland12. Detailed information on the SHCS is available on http://www.shcs.ch. The SHCS, founded in 1988, is highly representative of the HIV epidemic in Switzerland as it includes an estimated 53% of all HIV cases diagnosed in Switzerland since the onset of the epidemic, 72% of all patients receiving antiretroviral treatment in Switzerland, and 69% of the nationwide-registered AIDS cases12. The SHCS is registered under the Swiss National Science longitudinal platform: http://www.snf.ch/en/funding/programmes/longitudinal-studies/Pages/default.aspx#Currently%20supported%20longitudinal%20studies.
The ZPHI is a continuous, observational, non-randomized, single-centre cohort founded in 2002 that specifically enrols patients with documented acute or recent primary HIV-1 infection (https://www.clinicaltrials.gov/; ID NCT00537966)13.
Establishment of the transmission pair cohort
Overview
We established a cohort of 303 putative transmission pairs by screening for potential transmission pairs within a cross-sectional starting cohort of 4,281 chronic HIV-1-infected individuals included in the Swiss 4.5K Screen4,5. In addition to extensive patient demographic and clinical data, we had access to data on pol sequence, neutralization activity4 and HIV-1 binding antibody responses5,14 (Extended Data Fig. 1d) for these individuals.
We phylogenetically determined potential transmission pairs within the 4,281 patient starting cohort based on a threshold of pol gene similarity that was allowed to include individuals with a long infection history (Extended Data Fig. 1e, f and Supplementary Data 1). pol similarity has been previously established as reliable method to record genetic similarity of the infecting virus. Almost all larger molecular epidemiology work in HIV is based on HIV pol15,16,17,18,19. Moreover, owing to genetic linkage, similarity in pol and similarity in env are highly correlated in transmission pairs13,20,21. We determined potential transmission pairs as nearest neighbours (cherries) with a genetic distance of less than 0.045 on a pol phylogeny16,22 (Extended Data Fig. 1e, f and Supplementary Data 1). In total, we identified 303 potential transmission pairs and assigned transmitter and recipient status based on estimated infection dates. Individuals in transmission pairs were predominantly male, men who have sex with men and infected with subtype B (Supplementary Data 1 and Extended Data Table 1), reflecting the main drivers of domestic HIV-1 transmission in Switzerland4,12,13. Overall, the cohort of 303 transmission pairs did not differ in terms of duration of infection, neutralization breadth, virus load and peripheral CD4 T cell counts from the remaining patients of the starting cohort (Extended Data Table 1). Specific steps conducted in the establishment of the cohort are described in full in the following sub-sections.
Construction of HIV-1 pol gene phylogenies
Potential transmission pairs were defined based on HIV-1 pol gene phylogenies (as described in detail previously16,22) using pol nucleotide sequence data available in the SHCS database. In brief, these sequences stem from clinically or epidemiologically implicated genotypic resistance tests and, thus, are not derived from the same sampling time points as the plasma samples used for analyses of antibody responses.
We constructed pol phylogenies from 19,604 partial pol sequences from 10,970 different SHCS cohort participants, which included the 4,281 patients of the starting cohort (Extended Data Fig. 1d), and an additional 90,994 sequences from the Los Alamos database (http://www.hiv.lanl.gov/). These latter were included to decrease the chances of false-positive random clustering. We retrieved from the Los Alamos database all available, non-Swiss, pol sequences (region: 2,253–3,870) with a minimal length of 900 bp as of September 2014. Redundant control sequences (different sequence ID but identical nucleotide sequence) were deduplicated. For the SHCS patients, sequences with a minimum length of 250 bp for the protease gene and 500 bp for the RT gene were included. All sequences were initially aligned to a HXB2 reference genome (http://www.ncbi.nlm.nih.gov/nuccore/K03455.1) using MUSCLE23. Next, insertions relative to HXB2 and resistance mutations according to Stanford (http://hivdb.stanford.edu/) and International Antiviral Society—USA (https://www.iasusa.org/) lists were removed. In the following step, a generalized time-reversible model-based tree was constructed using FastTree24. The R package ‘APE’ version 3.1 was used for tree exploration and analysis25.
Definition of potential transmission pairs
Transmission pairs were defined as monophyletic pairs of the 4,281 starting cohort sequences on the pol phylogeny. We assumed that pairs with a cophenetic distance >4.5%, a commonly used threshold, clustered due to statistical and/or methodological artefacts (such as underrepresentation or even absence of rare genotypes in the background sequences). These pairs were therefore disregarded. We chose the relatively liberal threshold of pair distances of up to 4.5% as it best accommodates our cohort and the research questions addressed for several reasons. Owing to the study design of the Swiss 4.5K Screen, infection length varied between participants as one intent of this screen was to assess the influence of infection length on antibody development. Additionally, sampling time points for antibody testing and pol sequencing differ as the latter data were retrieved from clinically implicated genotypic resistance tests (see above). Short genetic distances in pol are associated with recent sampling times (Extended Data Fig. 1f). A strict distance criterion therefore bears the increased risk to exclude pairs in which plasma was sampled during prolonged chronic infection (at least 3 years of untreated infection), which we have previously shown to be associated with broad neutralization4. Thus, high genetic distances are a marker for the length of the within-patient evolution of the virus and associated with bNAb development, a main outcome of our study. A more liberal distance threshold therefore ascertains that the relevant patient population is included, maximizing the statistical power of our analysis. It is also important to note that, since we included a large number of background sequences, the detected monophyly is already a strong signal for the formation of a pair, irrespective of the actual genetic distance. We nevertheless verified the results of our study in sensitivity analyses using stricter selection criteria for potential transmission pairs, all of which confirmed the robustness of our observations (Extended Data Fig. 5).
Potential and confirmed transmission pairs
The attending physician confirmed that the bNAb transmission pair (T282 and R282) was a heterosexual couple living in a stable relationship in Switzerland, with a female-to-male transmission based on clinical data and self-reporting by the patients. Transmission of a HIV-1 subtype B infection from the female (North African origin) to the male partner (Asian origin) is further supported by a higher genetic pol diversity of the female partner (diversity = 0.53% for T282 and diversity = 0.20% for R282 on the same sampling date). On the basis of the available demographic data and infection timing, T282 infected R282 around 1.9 years post infection. The analysed plasma samples of the transmitter and recipient were collected 3.8 years and 3.4 years post infection, respectively. With the exception of T282 and R282, all other pairs should be viewed as potential transmission pairs as they possess genetically highly related virus strains in the pol phylogeny but have not been confirmed by alternative measures (physician records, self-reporting, and so on) and thus theoretically could also be partners in a tightly linked transmission cluster involving several people. For brevity we use the collective terms transmission pair(s)/transmission pair cohort without adding potential and/or confirmed to distinguish the respective patients. It is important to note that, as only the genetic relatedness of the infecting virus is of relevance for our study, neither the definition of confirmed pairs nor the tracing of the transmission time point is of relevance in the context of the conducted analyses.
Definition of transmitter and recipient within a pair
In a given transmission pair, we identified the individual with the earlier estimated infection date as the transmitter and the other as the recipient. In accordance with a previous study26, our results were, however, not affected by this assumption. The analyses shown in Fig. 1c, Extended Data Figs. 3b, c, 5d, e and Extended Data Table 2 are by necessity symmetrical (that is, insensitive) with respect to which patient is identified as transmitter and recipient. The analyses shown in Fig. 2a, b and Extended Data Figs. 4, 5a–c are not by necessity symmetrical, that is, they are potentially affected by which patient is identified as transmitter and recipient. We obtained, however, identical results when randomly assigning the role of transmitter and recipient within a transmission pair (Extended Data Fig. 3a). Note that this type of randomization does not change the grouping of patients into pairs but only which patient in a pair is considered transmitter or recipient.
HIV-1 binding antibody profile of the transmission pair cohort
The plasma IgG1, IgG2, IgG3 binding antibody reactivity to 13 HIV-1 Gag and Env antigens have been established for all 606 individuals in the 303 transmission pair cohort in a prior study analysing HIV-1 binding antibody of the 4,281 starting cohort5. See Supplementary Methods for details.
HIV-1 neutralizing antibody profile of the transmission pair cohort
Plasma neutralization activity of the 606 patients in the transmission pair cohort against a 14 multi-clade pseudovirus panel was determined as part of the current study. See Supplementary Methods for details.
Profiling of the neutralization breadth in the bNAb transmission pair T282 and R282
Prediction of bNAb epitope specificity in plasma bNAb of transmission pair T282 and R282
See Supplementary Methods and a previously published study27.
Strategies to determine the antibody-imprinting capacity of HIV-1
To investigate the similarity of antibody responses in transmission pairs, we used a series of approaches (summarized in Extended Data Fig. 2e and detailed below). In the context of our study, the strength of the overall effect of virus genetics on antibody responses measured by the above analyses is of secondary importance, as it can be the result of a strong influence of virus genetics in a few transmission cases and a weak/non-existent influence in most other cases within the cohort. Our analyses are thus tailored to provide proof of existence of an overall viral heritability, which—even if low—is a necessary condition for the search for bNAb imprinter viruses in a next step. The essence of what we investigate (see Fig. 1) is thus the similarity of the pattern of the responses across antigens/viruses and not that specific individuals have high antibody responses to all antigens/viruses.
Our analysis strategy followed three principle steps. First, we tested, for all 14 neutralization and 39 binding parameters, whether a given parameter is correlated within transmission pairs using Spearman correlations (ρSpearman for each parameter) (Fig. 1a and Extended Data Figs. 3a, 4a, c).
Second, the strength of the association is averaged across all neutralization, IgG1, IgG2 or IgG3 parameters to obtain a measure for the overall similarity of responses (average ρSpearman; Fig. 1b and Extended Data Figs. 4b, d, 5a–c).
Third, a mixed-effect Tobit model was used to estimate the fraction of the variance explained by viral genetic factors, which can in addition be adjusted for the effect of covariables (Fig. 1c and Extended Data Figs. 3b, c, 5d, e). A Tobit model was used because the neutralization percentage data are always non-negative and the binding data are approximately uniformly distributed within the range of 0–1. The 303 pairs constitute the groups used in the mixed-effect Tobit model. The model estimates three types of variances, the group-level variance σP2, the individual level variance σI2, and (if cofactors are included in the model) the variance explained by the cofactors σC2. Accordingly, the heritability is then given by
This constitutes a conservative approach to estimate heritability, since the variance explained by cofactors is also included in the denominator; that is, it is assumed to contribute to the non-heritable portion of the response although some cofactors (viral load, subtype and diversity) are at least partially steered by virus genetics. This approach is applied to each pseudovirus of the neutralization panel and each antigen separately and then averaged over all pseudoviruses/antigens in order to obtain an overall heritability estimate (Fig. 1c, Extended Data Figs. 3b, c, 5d, e and Extended Data Table 2).
In addition, we used linear mixed-effect models as an alternative method to derive heritability estimates, as these are commonly used26,28 and faster to be computed than Tobit models. The resulting estimates from variously adjusted linear mixed-effect models as well as standard errors derived from these models (by leave-one-out analyses) are compared to the Tobit estimates in Extended Data Fig. 3b. The standard errors proved to be small, and the linear mixed-effect models revealed almost identical effects to the Tobit mixed-effect models, highlighting the robustness of our findings.
In all three approaches, the statistical significance of a given heritability value (either for an individual pseudovirus or antigen, or averaged across pseudoviruses/antigens) is derived by comparing the observed value with the distribution obtained in 1,000 random reassignments of the recipients. The respective P value is then given by the inverse of the number of randomizations for which heritability is at least as high as in the original dataset. In Fig. 1b and Extended Data Figs. 4b, d, 5a–c, we consider two kinds of random reassignments: (1) completely random reassignment of recipients to transmitters and (2) random reassignment of recipients to transmitters with the same demographics (subtype (B versus non-B), ethnicity (white versus non-white), untreated infection length (1–3 years, 3–5 years, >5 years)). The latter adjusts for the potentially confounding effect of subtype, ethnicity and infection length. See also Supplementary Methods and previously published studies29,30 for details on how we controlled for potential confounders.
Single-genome amplification of the HIV-1 envelope
See Supplementary Methods and a previous study31.
HIV-1 envelope cloning from undiluted cDNA
Infusion vector cloning and sequencing
HIV-1 full-length genome sequencing and analysis
See Supplementary Methods and previously published studies32,33,34,35,36.
HIV-1 envelope phylogenetic analysis
See Supplementary Methods and previously published studies37,38,39.
Systematic strategy to trace HIV-1 strains with bNAb-imprinting capacity
To derive a method that allows a systematic identification of HIV-1 strains that have the capacity to induce (imprint) bNAb activity, we used a multi-step approach summarized in Extended Data Fig. 8.
Step 1. For each transmission pair, we test whether the antibody response across pseudo-viruses or antigens is correlated. This indicates whether the two members of a pair have high responses against the same viruses or antigens. Specifically, we determine the Spearman correlation coefficient of the neutralization responses in transmitter and recipient, and the same is done for the IgG1-binding response for each transmission pair. The two correlation coefficients are combined to obtain a single antibody response similarity index (½ρSpearman-neutralization + ½ρSpearman-IgG1-binding). Note, we only use IgG1 binding responses as these dominate natural HIV-1 infections and also provided the highest within-pair similarity (average ρSpearman = 0.19, Pshuffling < 0.001; Fig. 1a, b).
Step 2. Because a large fraction of patients exhibits weak responses against all tested pseudoviruses (148 out of 606 patients distributed over 127 pairs neutralize each of the 14 viruses at <20%, that is, neutralization score 0), and the comparison of their fingerprints is thus uninformative, this fingerprint-based approach had to be restricted to pairs in which both patients exhibit a certain level of neutralization strength (as measured by the neutralization score). For each transmission pair, we calculated the neutralization strength as the minimum neutralization score of the two individuals.
Step 3. Transmission pairs with highly similar antibody binding responses and high neutralization scores can now be identified (Fig. 3a, b).
Step 4. The number of transmission pairs with a similar (binding) and strong (neutralization) antibody response is determined for a broad range of similarity (0.3, 0.4, 0.5 and 0.6) and strength thresholds (1, 2, …, 7). To determine significance, these numbers were compared to those observed in 1,000 replicate datasets with shuffled transmission pairs, for which the shuffling is realized by assigning a randomly chosen recipient (sampling without replacement) to each transmitter (Fig. 3c, d).
For the interpretation of the results, it is important to note that not all pairs can be expected to show similar responses as in particular neutralization breadth is genuinely rare. In addition, in cross-sectional analyses as ours, it must be anticipated that occasionally the effects of the infecting virus are masked by the effect of differential infection length or other confounding factors in transmitter and recipient. We therefore control intensely for confounding factors (see also section ‘Strategies to determine the antibody-imprinting capacity of HIV-1’). The clear overall shift towards positively correlated responses (Fig. 3a, b), which is not a chance finding as we show (Fig. 3c, d), highlights that a considerable fraction of viruses exists that induce similar responses. Among these, rare cases with bNAb imprinting capacity are expected and can be screened for.
Reporting summary
Further information on research design is available in the Nature Research Reporting Summary linked to this paper.
Data availability
The antibody response and patient data reported in this paper are completely tabulated in Supplementary Data 1, 2. Sequence data of T282–R282 Env consensus and Env clones reported in Fig. 2c are deposited in GenBank. Accession codes are listed in Extended Data Fig. 6b. The raw sequencing files of the Illumina full HIV sequencing data of patients T282 and R282 referred to in Fig. 2c and Extended Data Fig. 6 have been uploaded to https://zenodo.org/ (https://doi.org/10.5281/zenodo.1324259). pol sequence data of the 606 studied cases are available from the corresponding authors and/or the SHCS scientific board (http://www.shcs.ch/contact) upon request.
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Acknowledgements
Financial support for this study has been provided by the Swiss National Science Foundation (SNF; 314730_152663 and 314730_172790 to A.T.; 324730B_179571 to H.F.G.; PZ00P3-142411 and BSSGI0_155851 to R.D.K.), the Clinical Priority Research Program of the University of Zurich (Viral infectious diseases: Zurich Primary HIV Infection Study to H.F.G. and A.T.), the Yvonne-Jacob Foundation (to H.F.G.), the Swiss Vaccine Research Institute (to A.T., H.F.G. and R.D.K.) and the SystemsX.ch grant AntibodyX (to A.T.). This study has been cofinanced within the framework of the Swiss HIV Cohort Study, supported by the SNF (33CS30_148522 to H.F.G.), by the small nested SHCS project 744 (to A.T.) and by the SHCS research foundation. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. The SHCS data are collected by the five Swiss University Hospitals, two Cantonal Hospitals, 15 affiliated hospitals and 36 private physicians (listed in http://www.shcs.ch/180-health-care-providers). We thank the patients participating in the ZPHI and the SHCS and their physicians and study nurses for patient care and D. Perraudin and M. Minichiello for administrative assistance.
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Nature thanks P. Lemey, J. Overbaugh and the other anonymous reviewer(s) for their contribution to the peer review of this work.
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R.D.K., P.R., C.K., H.F.G. and A.T. conceived and designed the study and analysed data. M.Hu., A.M., H.E., M.S., T.L., N.F., J.W., T.U., N.S.B., C.L., H.K., J.B. and K.J.M. conducted experiments and analysed data. D.L.B., A.U.S., J.-P.C., M.C., E.B., M.Ho., A.C., M.B., A.R., S.Y., V.A., T.K., H.F.G. and the members of the Swiss HIV Cohort Study conceived and managed the SHCS and ZPHI cohorts, collected and contributed patient samples and clinical data. R.D.K., C.K., M.S., H.F.G. and A.T. wrote the manuscript, on which all co-authors commented.
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The University of Zurich filed a European patent application (EP18184854.0) that includes the full envelope sequences of patients T282 and R282 or components thereof for use as bNAb-inducing immunogens with R.D.K., P.R., H.F.G. and A.T. listed as inventors. All other authors declare no competing interests.
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Extended data figures and tables
Extended Data Fig. 1 Selection and characterization of the HIV-1 transmission cohort used to investigate the antibody imprinting capacity of HIV-1.
a, b, Principal aims of the study. a, Defining the binding and neutralizing antibody imprinting capacity of HIV-1 strains/immunogens (that is, determining the heritability of these responses). The schematic depicts the possible outcomes of a transmission. The recipient may either have the same or a different type of antibody response as the transmitter. b, Creating means to identify bNAb-imprinting HIV-1 strains. The schematic depicts the possible outcomes of a transmission if the transmitter has a bNAb response. The recipient may also develop a bNAb response or not. c, Workflow of the study. d, The search for transmission pairs started with a cohort of 4,281 patients, who were included in the Swiss 4.5K Screen4 and for which HIV-1 antibody-binding data are available5. e, Histogram of the genetic (pol) distance of the 303 identified transmission pairs. f, Genetic (pol) distance to the transmission partner stratified by duration of untreated infection for the n = 606 patients in the transmission pair cohort. As in the Swiss 4.5K Screen, patients are grouped by infection length into categories of 1–3 years (n = 138), 3–5 years (n = 252) and more than 5 years (n = 216). Medians are shown (centre line), each box spans the IQR and each whisker extends to the most extreme value no more than 1.5× IQR from the box. More extreme values are shown as points.
Extended Data Fig. 2 Neutralization score analyses and strategies to determine the antibody-imprinting capacity of HIV-1.
a, Neutralization activity against a multi-clade 14-virus panel of all 606 transmitter and recipient plasma samples. Dashed horizontal lines at 20%, 50% and 80% and brackets display the thresholds used for the assignment of scores. On the basis of these data, each plasma–virus combination received a score of 0–3. The neutralization score of a plasma sample is the sum of the 14 individual scores against the panel viruses (0–42). Individual data points are shown as jittered circles. b, c, Distribution of neutralization breadth (b; P = 0.69) and neutralization scores (c; P = 0.40) in n = 303 transmitters and recipients (P values: two-tailed Wilcoxon signed-rank test). Medians are shown (centre line), each box spans the IQR and the whiskers extend to the 10% and 90% percentile. Individual data points are shown as jittered circles. d, Scatter plot of the neutralization score of recipients and transmitters for all 303 transmission pairs (Spearman; ρ = 0.139, P = 0.015). The number of pairs with the indicated values is depicted by dot size. e, Strategies to determine the antibody-imprinting capacity of HIV-1. For each of the 14 neutralization and 39 binding reactivities, the similarity in reactivity (Spearman correlation) was compared between transmitters and recipients to test whether transmission partners shared similar antibody responses.
Extended Data Fig. 3 Antibody similarity measurements are insensitive to the assignment of transmitter and recipient status, to choice of confounders and outliers.
a, Distribution of Spearman correlations (as in Fig. 1a) of neutralization–antibody-binding responses in pairs, in which the role of transmitter and recipient was randomly assigned within each of the n = 303 pairs (1,000 reassignments). Each violin plot is smoothed using a normal kernel, and its width represents the likelihood of a certain Spearman correlation. Grey daggers correspond to the similarities retrieved for the actual assignment of transmitter and recipient used in this study. For all investigated parameters, there was no statistically significant difference between the actual assignment and the shuffled assignment of transmitters and recipients (two-sided PSpearman > 0.05). b, Proportion of variability in responses explained by the infecting virus, determined using mixed-effect Tobit regression models (black circles) and linear mixed-effect models (horizontal bars). Standard errors of the linear mixed-effect models (black error bar; obtained by leave-one-out analyses) are shown. In each row, the models were adjusted for the indicated set of cofactors and only transmission pairs with complete information were included (number of pairs shown per row). c, Proportion of variability in responses explained by the infecting virus, determined using mixed-effect Tobit regression models on the full 303 pairs for which missing cofactors were imputed based on the other cofactors. Each violin plot is the result of 100 independent imputations, smoothed using a normal kernel, and its width represents the likelihood of a certain variability. Medians are shown (lines).
Extended Data Fig. 4 Similarity of neutralization and antibody-binding responses in subtype-B-infected transmission pairs.
a–d, To exclude influences of the subtype of the infecting virus, as a sensitivity analysis to Fig. 1a, b, the similarity of neutralization (a, b) and antibody-binding (c, d) responses was tested for the subset of subtype-B-infected transmission pairs (n = 254). a, c, Spearman correlation of the neutralization–antibody-binding response to each pseudovirus or antigen. Significant correlations (two-sided PSpearman < 0.05) are coloured. b, d, Average Spearman correlation of antibody responses in observed transmission pairs (n = 303) compared to two alternative scenarios: (1) completely random reassignment of recipients to transmitters and (2) random reassignment of recipients to transmitters with same demographics (subtype, ethnicity and untreated infection length). One-sided P values were derived from comparison with 1,000 reassignments. Each violin plot is smoothed using a normal kernel, and its width represents the likelihood of a certain average correlation in the respective alternative scenario. The medians are shown (white dots), each box spans the IQR and each whisker extends to the most extreme value no more than 1.5× IQR from the box.
Extended Data Fig. 5 Within-pair similarity of neutralization and binding responses remains significant for transmission pairs with lower genetic distance.
a–c, As a sensitivity analysis for Fig. 1b, the average similarity of neutralization and antibody-binding responses was determined for those transmission pairs with a genetic distance <0.03 (a, n = 280), <0.02 (b, n = 243) or <0.01 (c, n = 148), and compared to two alternative scenarios: (1) completely random reassignment of recipients to transmitters and (2) random reassignment of recipients to transmitters with same demographics (subtype, ethnicity and untreated infection length). One-sided P values were derived from comparison with 1,000 reassignments. Each violin plot is smoothed using a normal kernel, and its width represents the likelihood of a certain average correlation in the respective alternative scenario. The medians are shown (white dots), each box spans the IQR and each whisker extends to the most extreme value no more than 1.5× IQR from the box. d, e, As a sensitivity analysis for Fig. 1c, the proportion of variability in responses explained by the infecting virus, determined using unadjusted (d) and fully adjusted (e) (adjusted for duration of infection, subtype, ethnicity, log viral load and diversity) mixed-effect Tobit regression models is shown when restricting the analysis to closely related pairs (threshold on the x axis).
Extended Data Fig. 6 Full-genome comparison of T282 and R282 consensus sequences.
a, Multiple sequence alignment of the full genome consensus sequences of T282 and R282 with HXB2. Nucleotide variations from HXB2 are depicted by colour: A (red), T (green), C (blue), G (yellow); deletions by a horizontal bar. b, Overview and accession codes of env sequences derived from three bNAb-imprinting transmission pairs depicted in Fig. 2c. Indicated transmission time estimate is based on estimated time of infection of recipient.
Extended Data Fig. 7 Mutant virus neutralization mapping and distribution of transmission pair characteristics among pairs with and without transferability of antibody response.
a, Changes in neutralization activity of wild-type and mutant viruses were compared for six bNAbs (four targeting the CD4 binding site, two targeting the V3 glycan) and for the plasma of the elite-neutralizing pair. Increases in mutant half-maximum inhibitory concentration (IC50) values >tenfold and decreases in mutant half-maximum neutralization titre (NT50) values >two fold appear coloured. b, c, Association of transmission pair characteristics and transferability of antibody response in n = 303 transmission pairs. Transferability of antibody responses was determined according to relatively liberal (strength threshold = 4 and similarity threshold = 0.4) and strict criteria (strength threshold = 5 and similarity threshold = 0.5). b, Influence of continuous variables (mean log10 HIV-1 RNA in the transmission pair, the difference of these log10 RNA values, and the genetic distance in the pair) tested by univariable logistic regression. c, Influence of categorical variables (acute infection, long virus evolution, infecting subtype, ethnicity and transmission mode) tested by two-tailed Fisher’s exact test. The area of a rectangle corresponds to the number of pairs with the respective characteristic. MSM, men who have sex with men; HET, heterosexual transmission; IDU, intravenous drug users.
Extended Data Fig. 8 Systematic strategy to trace HIV-1 strains with bNAb-imprinting capacity.
HIV-1 strains that have the capacity to induce bNAb activity can be identified by measuring the similarity and the strength of the antibody response in each pair. A stepwise description of the approach is shown. See Methods ‘Systematic strategy to trace HIV-1 strains with bNAb-imprinting capacity’ for details.
Supplementary Information
Supplementary Methods
This file contains a Supplementary Methods, providing extended methods descriptions.
Supplementary Data
This file contains Supplementary Dataset 1: Patient characteristics, neutralisation and binding responses of the 606 patients in the transmission pair cohort.
Supplementary Data
This file contains Supplementary Dataset 2: Neutralization data of bnAbs and the elite-neutralizing transmission pair.
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Kouyos, R.D., Rusert, P., Kadelka, C. et al. Tracing HIV-1 strains that imprint broadly neutralizing antibody responses. Nature 561, 406–410 (2018). https://doi.org/10.1038/s41586-018-0517-0
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DOI: https://doi.org/10.1038/s41586-018-0517-0
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