Clinical examinations

A clinical examination was performed at screening, randomisation and certain follow-up protocol visits. At each visit the following data were recorded: body weight and height and all adverse events (AEs) since the last protocol visit, including in particular haematological abnormalities, pancreatitis, diarrhoea, clinical lipodystrophy, acute illnesses and change in HIV disease stage since the last protocol visit.

A physician assessment of lipodystrophy and Tanner stage was performed at week 0 and repeated every 24 weeks until the end of the study. A pregnancy test was performed for all females of childbearing potential at screening (weeks –4 to –2) and repeated every 24 weeks until the end of the trial and at other time points if required.

Ethnic-origin data were collected because it is known that ethnicity is a factor in the concentration levels of EFV.

Laboratory tests for efficacy and safety monitoring

• Haematology: haemoglobin, mean corpuscular red blood cell volume (MCV), platelets, white cell count, neutrophil and lymphocyte counts.
• Biochemistry: creatinine, albumin, total bilirubin, ALT, AST, alkaline phosphatase, calcium, phosphate.
• Lipids/glucose: triglycerides, cholesterol [total, low-density lipoprotein (LDL), high-density lipoprotein, very-low-density lipoprotein], glucose (participants should have been fasting overnight at randomisation, weeks 24 and 48 and then every 48 weeks during the main trial).
• Lymphocyte subsets: CD3 (absolute and percentage), CD3 + CD4 (absolute and percentage*), CD3 + CD8 (absolute and percentage*), total lymphocyte count (if measured by immunology laboratory) (*CD45RO/RA if measured).
• Virology: HIV-1 RNA (VL) using an ultrasensitive assay and resistance testing [locally or on stored samples (when VL was detectable)].

Screening visit

At the screening visit a trial number was assigned and used on all paperwork and labels. A clinical assessment was completed and the participant and/or carer completed an adherence questionnaire according to the young person’s age and knowledge of HIV diagnosis.

Blood was taken for haematological and biochemical investigations, for measurement of T-cell subsets (including RO/RA phenotype when available), for measurement of HIV-1 RNA VL (it was requested to use the same assay at least throughout the pilot phase and ideally throughout the whole trial, although the assays used varied across centres according to clinical practice and management) and for plasma and cell storage (at clinical centres where this was possible).

Randomisation visit

Randomisation (week 0) took place no more than 4 weeks after the screening visit and ideally as soon as possible after eligibility had been confirmed. The eligibility criteria and consent were reconfirmed verbally and noted on the randomisation form. Once a patient was randomised, a clinical assessment was completed, which included measurements of height and weight, presence of AEs, change in HIV disease stage and ethnic origin. The following investigations were performed: haematology, biochemistry, glucose and lipid profiles (fasting) and T-cell subsets (plus RO/RA phenotype if available). Blood was taken for plasma storage (plus cell storage if the participant attended a clinical centre where this procedure was possible or where a courier could be arranged). A quality-of-life questionnaire [Pediatric Quality of Life Inventory; see www.pedsql.org/ (accessed 6 April 2016)] was completed for all participants (and carers) and an acceptability questionnaire was completed for those young people randomised to SCT (and carers). Participants were given a diary to record when they took their ART, which included a reminder to restart therapy after the 2 days off ART in the SCT arm.

Follow-up

Young people were followed until the last randomised participant had completed 48 weeks of follow-up. All young people were seen for clinic visits at weeks –4 to –2 (screening), 0 (randomisation), 4, 12, 24, 36 and 48.

Primary end point

The primary analysis was performed on the intention-to-treat population. We used Kaplan–Meier techniques to estimate the proportion of young people failing in each arm by the 48-week assessment, adjusting for stratification factors: age range (8–12, 13–17 and 18–24 years) and recruitment from an African site. Using these proportions, we were able to estimate the difference in the proportion failing between arms and obtain a 90% CI around the difference, using bootstrap standard errors. This CI was used as an indicator of whether or not the results were consistent with the non-inferiority of SCT compared with CT. The non-inferiority margin was prespecified at 12% so that, if the upper bound of the 90% CI of the difference between arms (SCT – CT) was < 0.12, non-inferiority would be demonstrated.

The primary analysis was repeated but without adjusting for stratification factors. Additionally, an analysis was performed investigating the crude proportion of young people who experienced virological failure up to the end of the 48-week assessment.

Secondary end points

All analyses performed on the primary end point were repeated but instead considering the end point as a confirmed VL of ≥ 400 copies/ml.

Immunology, biochemistry and lipids were evaluated at each follow-up visit up to 48 weeks after randomisation by fitting normal regression models, adjusting for randomised arm and baseline value.

Changes in ART from SCT to CT at any point during the first 48 weeks of the trial for those randomised to SCT were summarised by reason for changing strategy. Changes in ART regimen were summarised by arm.

Major HIV-1 resistance mutations³⁹ at the point of VL failure or any time after VL failure were summarised for any VL failures in the first 48 weeks, overall and by drug class. CDC stage B and C events, as well as any deaths, were summarised by arm.

Measuring adherence was an important aspect of the analysis as we were attempting to see whether or not randomised strategies were being adhered to. We measured adherence to the protocol in two ways: first, through adherence questionnaires and, second, through a MEMSCap^™ Medication Event Monitoring System (MEMSCap Inc., Durham, NC, USA) substudy on a subset of 61 patients.

Acceptability questionnaires were summarised at baseline and week 48, and the comparison between what young people found difficult before the study and what they found difficult during the study was examined using McNemar’s test.

Safety

Grade 3 and 4 clinical and laboratory AEs were summarised by arm. The difference in rate of grade 3 and 4 AEs between arms per 100 person-years was calculated using Poisson regression (with a random effect for person) and the number of young people with any grade 3 or 4 AE was compared between arms using a Fisher’s exact test. The same analyses were performed for ART-related AEs, treatment-modifying AEs and serious adverse event (SAEs).

Rationale behind methods and markers selected

The blood volume that can be collected in children is limited, which was a major influence on the techniques selected for use in this study. In view of the global recruitment of the PENTA 16 trial, the assay selection was also influenced by its robustness to freezing at –80 °C for variable periods of time.

A panel of 19 biomarkers has been studied in several trials by the immunology laboratory at the UCL Institute of Child Health. Together they cover markers of inflammation (interleukin 1 receptor antagonist, C-reactive protein, tumour necrosis factor alpha, interleukin 10, interleukin 6, interleukin 8), cardiovascular injury (monocyte chemoattractant protein 1, angiopoietin-1 and -2, E-selectin, P-selectin, intercellular adhesion molecule 3, thrombomodulin, serum amyloid A, soluble intercellular adhesion molecule 1, soluble vascular cell adhesion molecule, vascular endothelial growth factor) and disordered thrombogenesis [d-dimer, tissue factor (TF)].

Methods

Blood was collected in ethylenediaminetetra-acetic acid (EDTA) and spun within 4 hours of collection at 1500 g (≥ 2500 rpm) for 15 minutes to separate cells from plasma. The supernatant was removed and placed in aliquots with a minimum of 500 µl of plasma in each cryovial. Samples were frozen at –70 °C immediately. Repeat freeze–thaw cycles were avoided.

All samples were transported to the Institute of Child Health during September 2014 and the assays were run in batches between October and December 2014. All standards were run in duplicate. Initial work within the laboratory showed that the coefficient of variance between duplicate samples was ≤ 10%. Given the small volumes of blood available and the cost of the plates, 95% of samples were run singularly, with 5% duplicated to ensure consistent intra- and inter-assay precision. The lower limit of detection, determined by the mean plus 2 standard deviations of the output signal of 10 blank samples, was calculated for each biomarker.

Meso Scale Discovery technique

A total of 17 biomarkers were analysed using Meso Scale Discovery^® (MSD) assays (Gaithersburg, MD, USA). MSD assays use an electrochemiluminescence detection method similar to a sandwich enzyme-linked immunosorbent assay (ELISA) technique. High-binding carbon electrodes in the base of microplates have a 10 times greater binding capacity than polystyrene. Electrochemiluminescent (SULFO-TAG) labels are conjugated to detection antibodies. Within the analyser, electricity applied to the plate electrodes causes light emission by the SULFO-TAG labels. Light intensity is then measured to quantify analytes in the sample. Multiple excitation cycles of each label amplify the signal to enhance light levels and improve sensitivity allowing ultrasensitive assays to be run [see www.mesoscale.com/technical_resources/our_technology/ecl/ (accessed 18 February 2015)].

Five MSD plates were used. Table 1 lists the plates with the biomarkers on each plate. Assays were conducted according to standard manufacturer’s protocols. Samples were read using the QuickPlex SQ analyser (MSD).

TABLE 1

List of biomarkers on each plate

Tissue factor

Tissue factor levels were measured using a commercial quantitative sandwich ELISA kit (Quantikine^® ELISA Human Coagulation Factor III/Tissue Factor R&D Systems, Minneapolis, MN, USA). A total of 100 µl of assay diluent was added to 96-well microplates precoated with a monoclonal antibody against human TF. Subject plasma was diluted twofold in Calibrator diluent RD5-20 (R&D Systems). The 100-µl standards and then 100-µl diluted subject plasma were added and incubated for 2 hours at room temperature on a horizontal orbital microplate shaker set at 600 rpm. The plate was manually washed four times using wash buffer and excess fluid was removed by tapping the plate on a paper towel before 200 µl of TF enzyme-linked polyclonal antibody conjugate was added. After a further 2 hours’ incubation the wash cycle was repeated and 200 µl of substrate solution [stabilised hydrogen peroxide/chromogen (tetramethylbenzidine)] was added. The plate was then protected from light during a final 30-minute incubation, after which 50 µl of stop solution was added, and optical density was measured within 30 minutes using a microplate reader (Thermo Scientific Multiskan^® EX) set to 450 nm. A four-parameter logistic curve fit was calculated using Ascent software 2.6 (Thermo Labsystems Oy, Basingstoke, UK) and the concentration read from the standard curve and multiplied by the dilution factor of two.

D-dimer

The commercial TECHNOZYM^® D-dimer ELISA assay (Technoclone, Vienna, Austria) was chosen following a comparison of two ELISA methods with two automated methods used in the NHS coagulation laboratory at Great Ormond Street Hospital. This provided consistent results and required smaller volumes of blood than the automated methods.

Undiluted samples were used after pilot runs showed that most patients had levels of D-dimer below the limit of detection when a twofold dilution was used. A total of 100 µl of calibrator and sample were added to wells precoated with anti-D-dimer monoclonal antibody and were then incubated at 37 °C for 60 minutes. Following manual plate washing three times using wash buffer (pH 7.3), 100 µl of conjugate (monoclonal Anti D-dimer-POX) working solution was added before a further 60-minute incubation at 37 °C. Following a second plate wash, 100 µl of substrate solution (chromogen tetramethylbenzidine) was added. After a 10-minute incubation at room temperature, 100 µl of stop solution (sulphuric acid) was added and the plate read immediately using a microplate reader (Multiskan EX) set to 450 nm. A linear regression curve fit was calculated using Ascent software 2.6 and the concentration read from the standard curve.

Statistical methods

Two linear regression models were fitted for each biomarker, at 48 and 96 weeks, adjusting for baseline biomarker value and randomised arm. However, because of the non-normal distribution of each biomarker, the natural logarithm was used to fit the models.

Rationale for an immunology substudy

A study comparing CD4-guided planned treatment interruptions of ART with CT in HIV-1-infected children was performed between 2004 and 2006.⁴⁰ The key immunological findings were that (1) there was a rapid fall in CD4 cells that occurred early following treatment interruption; (2) there was a rapid increase in CD8 cells peaking at 8 weeks after the planned treatment interruption; and (3) there were changes in naive and memory cell subsets within both the CD4 and the CD8 cell populations.⁴¹ This study informed our focus on these cell populations to determine whether or not treatment interruption in the BREATHER trial would have an impact on immune dynamics.

Methods

The CD4 and CD8 lymphocyte subsets were quantified locally on fresh samples collected. In some centres, CD45RA and CD45RO subpopulations of CD4 and CD8 cells were also evaluated on fresh samples. In centres able to separate and store cells, additional whole blood was collected in EDTA and peripheral blood mononuclear cells isolated by density gradient centrifugation, divided into aliquots and frozen. A range of established markers was used to quantify naive and memory cells. These varied between laboratories but always included antibodies to detect CD45RA and CD45RO; in some laboratories, CD27 and CD31 were also included.

Statistical methods

Linear models of the CD45RA/CD45RO ratio, adjusting for baseline CD45RA/CD45RO ratio and randomised arm, were fitted at 48 weeks. Similar models were fitted for CD45RA%/CD45RO%, CD8RA/CD8RO and CD8RA%/CD8RO%. Because of non-normal distributions of these ratios, the natural logarithm of each ratio was used to fit the models.

Statistical methods

We compared the proportion of individuals at week 48 with a VL of ≥ 20 copies/ml with the proportion with a VL of ≥ 50 copies/ml from the main trial analysis. Additionally, we investigated the difference between arms in the proportion of young people with a VL of ≥ 20 copies/ml at week 48 and tested the difference using a Fisher’s exact test.

We examined how many individuals who failed during the first 48 weeks of the main trial had a screening (or baseline if no screening sample available) VL of ≥ 20 copies/ml.

Finally, we compared the proportion of young people in each arm who had a VL of < 20 copies/ml at screening (or baseline if no screening sample available) and a VL of ≥ 20 copies/ml at week 48 using a Fisher’s exact test.

Laboratory methods

Sample

All young people recruited into the BREATHER trial in the UK, Ireland, Uganda and the USA aged 10–24 years were eligible to participate in the qualitative substudy, subject to the appropriate consents and self-awareness of HIV infection (for at least 6 months). Although the trial included children from the age of 8 years, the qualitative study involved trial participants who were aged ≥ 10 years only and aware of their HIV status. Although we appreciate that age can be an inadequate proxy for HIV awareness, this decision was guided by ethical concerns about the extent to which children under the age of 10 years could have achieved the considerable understanding about HIV infection necessary for the in-depth discussions in the qualitative interviews.

In our design we had envisaged that we would adopt a purposive sampling strategy giving primary emphasis to ‘responsibility for medication’ (sole, shared, carer), with secondary dimensions including age (spread as per trial), gender, ethnicity, membership of HIV youth support groups, current domestic situation (living with parent(s), extended kin) and school attendance. However, given the lower than expected levels of recruitment into the trial in the UK and Ireland, we involved anybody who was eligible and willing to participate. In the US site, given the nature and timing of the fieldwork we adopted the same strategy, which meant that we involved all participants who had thus far been recruited into the trial. In Uganda, excluding those who were in the pilot, we initially adopted a similar recruitment strategy as in the other sites and then purposively selected the last 10 in our sample to ensure that we were reflecting a broad range of sample characteristics. The qualitative sample in each site reflects the diversity of the trial population.

Overall, 102 interviews were conducted with 43 young people (Table 2). In total, 26 young people were recruited in Uganda from one clinic (Joint Clinical Research Centre, Kampala), seven were recruited in the UK from three clinics (NHS hospitals in London, Nottingham and Dublin) and 10 were recruited in the USA from one clinic (St. Jude’s Children’s Research Hospital, Memphis, TN).

TABLE 2

Qualitative sample overview

Recruitment response and retention through the repeated phases of the qualitative study was high (around 40%). We had very high rates of participation in the Uganda (26 out of a possible 66 trial participants) and US sites (10/14). Recruitment was most challenging in the UK and Ireland (7/23). Overall, we included 40% of the trial participants who were aged ≥ 10 years. However, the actual proportion of eligible participants recruited is likely to have been higher than this, given that this figure does not account for the participants who would not have been eligible despite being within the age range because of a lack of awareness of their HIV status.

The majority of refusals occurred in the UK sites, with the reasons for refusal varying. Very few participants had taken part in qualitative research before and some of the young people were unwilling to talk to the researchers and were uncomfortable with the idea of the qualitative interviews. Others instead mentioned not wanting to take on any additional clinic attendance and time commitments. This may reflect the amount of overall research being conducted with the relatively small UK cohort, but could also be indicative of the desire that young people have to minimise the time spent in the clinic and focus on other aspects of their lives aside from HIV.

Types of data collected

1. One-to-one interviews with young people living with HIV. In Uganda, participants were interviewed three times over the course of the study (in the early stages of the trial; towards the end of the trial; and during the follow-up period) to explore their experience of adherence and the process of the trial. In the UK and US sites, only the first two interviews were conducted. Interviews lasted approximately 1–2 hours and were audio-recorded, subject to consent. Baseline interviews captured life with HIV on HIV treatment as described by young people and included, but did not focus specifically on, young people’s perceptions of the trial or of SCT. The second interview reconstructed the life and treatment trajectory of participants since the start of the trial, focusing on adherence during this specific time period as well as reflections on intervention and trial acceptability. The third interview in Uganda was conducted as participants moved into the follow-up stage of the study. In these interviews we explored any changes in their treatment experience and their attitudes towards continuing in the intervention or control arm. The third interviews are being conducted in the UK only at trial end to explore participants’ reactions to the outcome of the trial. Reactions to the trial results will be explored informally in Uganda through meeting observations and discussions. It is worth noting that the focus of the third interview has changed from the preliminary study design in response to the changes made in the trial. The third interview was initially planned to explore how participants would adapt had they been required at the end of the trial to switch back from the SCT arm to CT. However, this has not occurred and participants have been retained in the same arm through the follow-up phase. The focus of the qualitative enquiry has shifted to reflect these changes and instead will consider how participants respond to continuing in the same arm and their attitudes towards SCT once the main trial findings have been disseminated.
2. Audio diaries of young people living with HIV. We piloted the use of audio diaries in the UK and Uganda sites. This is an innovative method that we have used before and we consider such diaries to be a valuable method in capturing personal reflections.⁴² We wanted to explore whether or not this method would enable participants to generate data at the time and space of their choosing and if this would provide particular insights into the immediacy and variability of treatment and adherence experiences. We therefore offered this method to assess its feasibility and value for research with young people. All participants were offered the chance to keep an audio diary in the Uganda and UK sites. Ethical approval was not given for the audio diaries to be used in the US site. In Uganda, 12 participants agreed to contribute a personal audio diary and in the UK three participants took up the opportunity. We found that there were significant challenges to using audio diaries with this age group in these sites for such a sensitive topic. Despite participants’ initial enthusiasm to use the diaries we found that their lack of privacy within their own home, exacerbated for many (especially those in Uganda) by a lack of physical space, meant that it was difficult for them to first record their diaries with ease and second be confident of securely storing them before returning them to the research team. These conditions undermined the value of the method, as the premise that participants may be able to speak more freely about immediate events with greater convenience could not be realised. Those who did record something mainly recorded public interactions or songs, which were not related to our topic of enquiry. We may conclude from this pilot that use of audio diaries is unlikely to be a feasible method given the restraints of a lack of privacy.

Ongoing research: planned data collection

1. Phase 3 interviews with young people in the trial in the UK post publication of trial findings. In the UK we are conducting a third and final interview which explores attitudes towards SCT in light of the trial findings. Our research focus has been adjusted to reflect the trial plans. It remains rare for participants to be asked about their response to trial findings and we anticipate that this may provide a valuable model for informing the design of any further development of this intervention and future roll-out.
2. Interviews with carers of young people in the trial (Uganda). In Uganda, all participants have been asked to consent to their carers being contacted to take part in an interview. Using thematic sampling criteria, informed by our initial analysis, we are inviting 15 carers to participate in an interview to explore their response to the trial findings. The interview also explores their decision-making process in consenting for their child to participate in the trial, their reflections on how their expectations aligned with their experience of the trial and their perceptions of the barriers to and facilitators of adolescents’ adherence, including the impact of the trial.
3. Focus groups with young people living with HIV not involved in the trial. In Uganda data are being collected in focus groups with up to 25 HIV-positive young people aged 10–24 years who participated in the trial. This is subject to the appropriate consents and self-awareness of HIV infection (for at least 6 months). These focus groups explore young people’s understandings of the results of the trial, their experience in the trial and its influence as their adherence patterns, through peer discussion. We endeavour to ensure that these groups reflect the diversity of the trial population. Data transcription and, where appropriate, translation from these additional sets of data collection are ongoing. Data analysis is being carried out iteratively to inform subsequent data collection and refine questions.

Consent procedures and ethics

Consent was sought from all trial participants aged 10–24 years who had been aware of their status for at least 6 months. Participants were approached in different ways depending on the local procedures of each of the research sites. In the UK, research nurses contacted and consented participants, although the researcher had a number of conversations over the telephone with participants to answer their questions and discuss the topic before they decided whether or not to take part. In the USA, trial staff carried out both the contacting and the consent procedures. In Uganda, the researcher met the carers in the clinic and explained the qualitative study to them and then asked for their consent for the children to participate. This was followed by an ‘assent’ procedure with the children themselves. In all sites, final arrangements for the interviews were organised with the researcher.

In line with Good Clinical Practice principles [see www.ich.org/products/guidelines/efficacy/efficacy-single/article/good-clinical-practice.html (accessed 6 April 2016)], informed consent was treated as a process. This involved reminding participants at each stage of the study what the qualitative study was about, answering any related questions that they may have had, providing information as appropriate and reiterating that participants could withdraw at any time during the process of data collection. We did not need to break confidentiality on any safeguarding issues, although we had plans in place should this have been necessary.

The data that were collected were transcribed verbatim and, when appropriate, were translated into English by the research assistant. Personal identifying details were removed. We have been given an exemption from the mandatory request by the Economic and Social Research Council to archive the Ugandan data given the sensitivity and contextually dense nature of the data collected.

Modes of analysis/interpretation

The study adopted a grounded analytic approach to thematic analysis, using systematic case comparison and negative case analysis throughout.⁴³ We orientated analyses by themes emerging within/across individual accounts, exploring the acceptability of the trial; the potential value of SCT; and barriers to adherence as it converges with changing priorities during adolescence, as well as to the advancement of social science research and theory on HIV treatment adherence.

All interviews and audio diaries were transcribed verbatim by the data assistants. As discussed above, the limitations in the audio diary data meant that these data have not been integrated into our analysis. In line with our iterative analysis approach, we analysed data as we collected it to inform the direction of subsequent interviews, further coding and case selection. In addition to giving attention to ‘negative cases’ through case comparisons in our analysis, we sought respondent validation on emerging conclusions and maximised internal reliability and reflection through comparing coding between multiple researchers. Coding was undertaken in two linked phases. Our first-level coding drew on a combination of a priori themes reflected in the study topic guide and inductive or in vivo codes.⁴⁴ Our second-level coding sought to break down first-level coded data into smaller units, which also involved moving from codes that operate at the level of participant description and meaning to concept-driven categories. This process is similar to moving from ‘open’ to ‘axial’ to ‘selective’ coding in grounded theory.⁴³ We have maintained an audit trail of the analytical process, including analytical memos and how case comparisons and attention to emerging negative cases have informed ongoing analyses. We have conducted analysis by site and across the study to identify if gender, age and country are significant in how we can disaggregate our findings.