key: cord-296277-paqu1t1e
authors: Fragaszy, Ellen B; Warren-Gash, Charlotte; Wang, Lili; Copas, Andrew; Dukes, Oliver; Edmunds, W John; Goonetilleke, Nilu; Harvey, Gabrielle; Johnson, Anne M; Kovar, Jana; Lim, Megan SC; McMichael, Andrew; Millett, Elizabeth RC; Nazareth, Irwin; Nguyen-Van-Tam, Jonathan S; Tabassum, Faiza; Watson, John M; Wurie, Fatima; Zambon, Maria; Hayward, Andrew C
title: Cohort Profile: The Flu Watch Study
date: 2016-03-03
journal: Int J Epidemiol
DOI: 10.1093/ije/dyv370
sha: 
doc_id: 296277
cord_uid: paqu1t1e

nan

Influenza is a common, highly contagious respiratory virus which infects all age groups, causing a range of outcomes from asymptomatic infection and mild respiratory disease to severe respiratory disease and death. 1 If infected, the adaptive immune system produces a humoral (antibody) and cell-mediated (T cell) immune response to fight the infection. 2 Influenza viruses continually evolve through antigenic drift, resulting in slightly different 'seasonal' influenza strains circulating each year. Population-level antibody immunity to these seasonal viruses builds up over time, so in any given season only a proportion of the population is susceptible to the circulating strains. Occasionally, influenza A viruses evolve rapidly through antigenic shift by swapping genes with influenza viruses usually circulating in animals. This process creates an immunologically distinct virus to which the population may have little to no antibody immunity. The virus can result in a pandemic if a large portion of the population is susceptible and the virus is easily spread. 1 International influenza surveillance is typically based upon cases seeking medical care. [3] [4] [5] However, this focus greatly underestimates the true community burden of seasonal influenza: the majority of cases are mild and self-limiting, with asymptomatic infections accounting for 25% to 75% of all infections. 6, 7 Effective influenza control requires knowledge of disease burden and factors affecting influenza transmission. Existing parameters for mathematical models of influenza interventions are largely derived from household cohort studies conducted in the USA between 1948 and 1981. [8] [9] [10] Since then there have been profound social changes affecting population contact and mixing patterns that are likely to impact on influenza transmission. These changes include more women working, more children attending day care, more commuting and international travel and increased vaccine coverage. Evolutionary changes to circulating viruses may affect transmission dynamics, patterns of clinical illness and the adaptive immune responses elicited. 1, 11 Rapid advances in laboratory methods have also occurred, providing unique opportunities to investigate immune correlates, both humoral and T cell based, with influenza infection rates and disease severity. 11, 12 The initial Flu Watch cohort, funded by the UK Medical Research Council (MRC), began in 2006 as a collaboration between epidemiologists at the Centre for Infectious Disease Epidemiology at University College London (UCL), virologists and mathematical modellers from the Health Protection Agency (HPA, now Public Health England), immunologists at the MRC Human Immunology Unit at Oxford University and the MRC General Practice Research Framework (GPRF). It aimed to estimate community burden of influenza and influenza-like illness, generate up-to-date knowledge of demographic, social and behavioural factors affecting influenza transmission, measure antibody and T cell immune responses to influenza and to use knowledge generated to inform modelling parameters. In addition, a pandemic preparedness cohort was envisioned, in which participants already familiar with the study consented to be re-contacted in the event of a pandemic, to allow rapid redeployment of the study.

When the 2009 influenza AH1N1 pandemic arose, further funding was secured jointly from the MRC and Wellcome Trust, allowing continued follow-up and an expansion in cohort size. New collaborators for this phase included the MRC Centre for Outbreak Analysis and Modelling, the Wellcome Sanger Institute, the Primary Care Research Network and additional epidemiology and public health experts from the HPA. Additional study aims were to inform the national and international response to the current and future pandemics. Specific objectives were to examine clinical profiles of illness, estimate population infection denominators and case fatality risk, describe epidemiological characteristics of the infection in real-time, monitor changes in population behaviour, and investigate access to services, attitudes to and uptake of antivirals and vaccine, and immunity to infection in order to inform vaccination policy and development. During the pandemic, Flu Watch also provided control data and samples for studies of severe influenza (MOSAIC) and studies of influenza infection risk in people working with pigs (COSI). 13, 14 Who is in the cohort?

Households were recruited from registers of 146 volunteer general practices (GP) across England, who formed part of the MRC GPRF or (from the 2009 pandemic onwards) the Primary Care Research Network. Participants were selected from GP lists by computer-based random number generation. GPs sent invitation letters inviting the randomly selected person and their household to participate. Although it was recognized that this would bias invitations towards larger households, such as those with children, this was accepted as the role of children in influenza transmission was an important research question. Weighting by the inverse of household size in analyses was planned to account for this sampling design.

To be eligible to participate, the whole household had to agree to take part in follow-up over the coming winter, with adults aged 16 years agreeing to have blood samples taken. Exclusion criteria included household size > 6 people, individuals with terminal illness, severe mental illness or incapacity and heavy involvement in other ongoing research. GPs reviewed invitation lists and removed anyone meeting these criteria, before sending letters. Cohorts were recruited to allow follow-up of participants over six influenza seasons-the 2006/07, 2007/08 and 2008/09 periods of seasonal influenza circulation, the summer and winter waves of the 2009 pandemic and the first post-pandemic season 2010/11. From season 3 (2008/09) onwards, previous participants were invited to take part again.

In season 1, invitation letters were sent to 2300 households from 42 practices, and 602 individuals from 243 households agreed to participate. In subsequent seasons the response rate was not monitored as practices (rather than the university study team) sent the invitation letters and not all returned data on numbers sent. Compared with the English population, young adults, non-White ethnic groups, people living in socially deprived areas and those living in the North of England, West Midlands and London were under-represented in the Flu Watch cohort (Table 1) .

The basic cohort design Baseline/pre-season phase A baseline visit was made to the household at enrolment, during which a research nurse collected blood samples for serological and T cell analysis from all adults aged 16 years or older. Blood sampling was optional for those aged 5-15 years and not done in those under 5 years of age. Visits occurred in the evenings, as bloods had to be couriered overnight to Oxford for early morning analysis of T cells. The serum samples collected we recentrifuged, frozen and later batch-tested for influenza antibodies by the HPA. Nurses assisted families with a series of laptop-based surveys collecting information on basic demographics, health and chronic illness, respiratory hygiene, household structure and relationships, accommodation, contacts and activities. Households received participant packs containing paper illness diaries, thermometers and nasal swab kits including instructions on their use and the viral transport medium to be stored in the refrigerator.

In order to obtain reliable measures of the number of illnesses, we actively contacted participants every week with automated telephone calls to assess the presence or absence of respiratory illness in each household member. For each respiratory illness, participants were reminded to fill in a prospective paper illness diary. These collected information on illness onset date, temperature and presence and severity of symptoms such as feeling feverish, headache, muscle aches, cough and sore throat. Diaries also collected data on contact patterns and activities before and during illness. Participants took a nasal swab on day 2 of any respiratory illness for polymerase chain reaction (PCR) analysis of influenza, respiratory syncytial virus (RSV), human metapneumovirus (hMPV), rhinovirus, coronavirus, adenovirus and parainfluenzavirus. During the first season, swabbing was limited to periods of influenza circulation. The Sanger Institute genetically sequenced some of the viral isolates from the summer and winter waves of the pandemic (seasons [4] [5] .

In addition, all participants completed one-off activity and contact paper diaries on at least 1 pre-determined weekday and 1 weekend day during the active follow-up period. These diaries collected information on where participants were (i.e. at home, at work etc.), whether they had contact with crowds and the number, duration and age groups of personal contacts throughout the day.

At the end of follow-up, nurses made a final household visit to take a follow-up blood sample (for paired serology) and assist participants with an exit survey. Nurses also checked participants' medical records for information on chronic illnesses, influenza and pneumococcal vaccinations, prescriptions, GP consultations, hospitalizations and deaths.

The cohort evolved over time to maximize system reliability, minimize the number of data sources and allow increased recruitment during the pandemic. In season 3 we offered participants the option of moving from paper illness diaries with weekly automated phone calls to weekly emailed surveys with or without optional SMS reminders.

For the pandemic and post-pandemic cohort, most surveys moved to a custom-built website for self-completion. In order to achieve real-time monitoring of illnesses during the pandemic, participants were emailed a link to a retrospective online weekly survey and provided with laminated wipe-clean charts at home to record daily symptoms as a memory aid. In season 3 there were additional one-off surveys collecting data on indoor and outdoor temperature and humidity, travel patterns and non-response to weekly surveys. During seasons 5 and 6 we added questions to existing surveys on attitudes towards influenza vaccination and antivirals. In season 6 we included quality of life questions. 15 

The cohort design evolved with the emergence of the novel H1N1 pandemic strain during season 3.We continued active follow-up through the UK summer wave of the pandemic (season 4). For the UK winter wave of the pandemic (season 5), the study split into three separate cohorts: T cell (comprising both previous and newly recruited participants), Serology and Virology (both comprising new participants). For the T cell cohort, continuing participants used the spring blood sample from season 3 as a baseline sample. They also gave a pre-vaccination blood sample to allow distinction of antibody rises caused by infection rather than vaccination. This was particularly important for the winter wave of the pandemic, as we anticipated widespread vaccination. The Serology cohort was identical but lacked T cell samples. For the Virology cohort, no blood samples were taken. This allowed for rapid recruitment of a large number of participants (n ¼ 1778) to increase the accuracy of weekly estimates of illness rates during the pandemic, with minimal nurse time required. All nasal swabs were tested for influenza A and B, RSV and hMPV but, due to the large number of samples generated during the pandemic, only a selection in seasons 5 and 6 were tested for other viruses.

Retention of enrolled participants throughout the cohorts was good. Figure 1 displays the number of enrolled participants each week, with arrows pointing out the staggered starts and exits of the cohorts along with other important dates. Loss to follow-up came in two main varieties: nonresponse to weekly contact and loss to follow-up for paired blood samples.

We obtained weekly responses from 87.3% of followup weeks overall, which increased to 88.4% if we exclude periods when there were technical difficulties with our automated phone calls (1 week in season 1 and 4 weeks in season 2). Response completeness generally increased after the introduction of email and online surveys in season 3 ( Table 2 ). Only 12.4% of households were classified as poor responders (responding to < 70% of follow-up weeks). Poor response appeared to be more common as deprivation increased.

We obtained paired blood samples from 80% of participants required to provide them and from 27% of participants aged 15 and under, for whom blood samples were optional (Table 3) .

The three main clinical outcomes were: (i) influenza-likeillness (ILI), defined as a respiratory illness with cough and/or sore throat and fever > 37.8 C;(ii) PCR-confirmed influenza illness; and (iii) influenza seroconversion, defined as a 4-fold titre rise in strain-specific antibody titres in unvaccinated individuals. Table 4 summarizes the data and biological samples collected during baseline, active follow-up and post-season phases. We additionally linked participants' data to small area statistics such as the index of multiple deprivation and rural/urban indicators. 16, 17 Details of the T cell methodology have been described previously. [18] [19] [20] What has been found? Key findings and publications Our first publication provided comprehensive national estimates of clinical and sub-clinical disease burden in the community regardless of consultations, and allowed comparison between seasonal and pandemic influenza. 2 We found that on average, influenza infected 18% of unvaccinated people each winter and up to 75% of these infections were asymptomatic. Approximately 25% of infections were PCR confirmed and only 17% of people with PCR-confirmed disease sought medical attention; Figure 2 indicates how the primary care-based surveillance underestimated the burden of infection in the community. Results were similar between pandemic and seasonal influenza, although people infected with the 2009 pandemic strain had less severe symptoms than those infected with seasonal H3N2 strains.

Our second publication provided strong evidence that naturally occurring, cross-protective T cell immunity protects those infected with influenza against developing disease in seasonal and pandemic periods. 16 This protection was independent of baseline antibodies and protective levels of influenza-specific T cells were found in 43% of the population. These findings help explain why such a large proportion of infections remain asymptomatic and have implications for the development of cross-protective 'universal' vaccines based on this response.

In order to evaluate different methods of collecting data during a pandemic, we compared prospectively collected Flu Watch data on illnesses and vaccine uptake with retrospectively collected data from the Health Survey for England. 21 We found that retrospectively collected data underestimated disease burden but accurately estimated vaccine uptake when compared with prospectively collected data.

Current work includes an analysis of occupational exposure to pigs as a risk factor for human infection with swine and human influenza viruses; age as a predictor of T cell responses; and a comparison of serological pandemic infection rates from Flu Watch and the Health Survey for England. We believe the poor response in this season may be due to summer holidays.

What are the main strengths and weaknesses?

Flu watch is a large community cohort study broadly representative of the population of England. It is the first modernday household study of influenza transmission in a temperate climate, comparable to the landmark Tecumseh studies of the 1960s and 70s. 22 A major strength is the inclusion of different household types (rather than just households with children, as in earlier studies) which allows influenza infections to be explored across the whole of society. We used highly active methods of surveillance for influenza and other respiratory 23 or from populations with high vaccination rates which greatly limits interpretation (1968 H3N2 pandemic). 22 Historical data on laboratory-confirmed rates of seasonal influenza mainly come from historical community studies of families in the USA between 1948 and 1981. 10, 22, 24, 25 Flu Watch is a good example of collaboration between disciplines (epidemiology, immunology, virology and primary care) and partners. The study provides a rich source of data on social, behavioural and biological factors affecting influenza transmission, enabling exploration of many research questions. Limitations include delays in obtaining funding, ethics and R&D approval across multiple sites, resulting in delayed recruitment during the pandemic and fewer participants overall. Although the initial response to invitation letters was low, it is unclear if this would bias results. Ideally, cohorts would have had pre-and post-influenza season bleeds, but recruitment periods were not perfectly streamlined with influenza seasons so adjustments for bleed timings were made during analysis. The study design and data collection methods evolved in response to experience and changing questions. Whereas this optimized and streamlined methods, it also increased complexity of data management.

Can I get hold of the data? Where can I find out more generate novel data on antibody and T cell immunity, to inform influenza control initiatives.

• A total of 5484 participants were recruited from 2205 households randomly selected from registers of participating general practices. 

Comparative community burden and severity of seasonal and pandemic influenza: results of the Flu Watch cohort study

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Seattle Virus Watch 4. Comparative epidemiologic observations of infections with influenza-A and influenza-B viruses, 1965-1969, in families with young children

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We acknowledge the contribution of Alison Bermingham, now sadly deceased, of the Respiratory Virus Unit, Centre for Infections, Public Health England. We thank all Flu Watch participants and nurses for their support of the study.

Peripheral blood mononuclear cells (PBMC) separated, part of the sample was immediately tested against pools of peptides representing each of the virus proteins in an ex vivo IFN-celispot assay. 18, 19 The rest of the sample was frozen down for more detailed peptide mapping studies using IFN-celispots and/or in vitro culture and testing by intracellular cytokine staining to determine CD8/4 restriction. Post-season T cell analysis was only conducted in seasons 1 and 3.