Clinical and laboratory evaluation of SARS-CoV-2 lateral flow assays for use in a national COVID-19 seroprevalence survey

Flower, Barnaby; Brown, Jonathan C.; Simmons, Bryony; Moshe, Maya; Frise, Rebecca; Penn, Rebecca; Kugathasan, Ruthiran; Petersen, Claire; Daunt, Anna; Ashby, Deborah; Riley, Steven; Atchison, Christina; Taylor, Graham P.; Satkunarajah, Sutha; Naar, Lenny; Klaber, Robert; Badhan, Anjna; Rosadas, Carolina; Khan, Maryam; Fernández, Natalia; Sureda-Vives, Macià; Cheeseman, Hannah; O’Hara, Jessica; Fontana, Gianluca; Pallett, Scott J C; Rayment, Michael; Jones, Rachael; Moore, Luke; McClure, Myra O.; Cherepanov, Peter; Tedder, Richard S.; Ashrafian, Hutan; Shattock, Robin J.; Ward, Helen; Darzi, Ara; Elliot, Paul; Barclay, William; Cooke, Graham

doi:10.1136/thoraxjnl-2020-215732

“…130 However, in the UK, nationally validated assays have been evaluated with convalescent samples from community participants and a number of large-scale serosurveys now use these. [131][132][133] Clear understanding of the kinetics of the response, particularly for the specific N and S antigens, is important for the interpretation of seroprevalence studies.…”

Section: Implications For Policymentioning

confidence: 99%

Antibody response to SARS-CoV-2 infection in humans: a systematic review

Post

¹

,

Eddy

²

,

Huntley

³

et al. 2020

Preprint

View full text Add to dashboard Cite

Introduction Progress in characterising the humoral immune response to Severe Acute Respiratory Syndrome 2 (SARS-CoV-2) has been rapid but areas of uncertainty persist. This review comprehensively evaluated evidence describing the antibody response to SARS-CoV-2 published from 01/01/2020-26/06/2020. Methods Systematic review. Keyword-structured searches were carried out in MEDLINE, Embase and COVID-19 Primer. Articles were independently screened on title, abstract and full text by two researchers, with arbitration of disagreements. Data were double-extracted into a pre-designed template, and studies critically appraised using a modified version of the MetaQAT tool, with resolution of disagreements by consensus. Findings were narratively synthesised. Results 150 papers were included. Most studies (75%) were observational in design, and included papers were generally of moderate quality based on hospitalised patients. Few considered mild or asymptomatic infection. Antibody dynamics were well described in the acute phase, and up to around 3 months from disease onset, although inconsistencies remain concerning clinical correlates. Development of neutralising antibodies following SARS-CoV-2 infection is typical, although titres may be low. Specific and potent neutralising antibodies have been isolated from convalescent plasma. Cross reactivity but limited cross neutralisation occurs with other HCoVs. Evidence for protective immunity in vivo is limited to small, short-term animal studies, which show promising initial results in the immediate recovery phase. Interpretation Published literature on immune responses to SARS-CoV-2 is of variable quality with considerable heterogeneity with regard to methods, study participants, outcomes measured and assays used. Antibody dynamics have been evaluated thoroughly in the acute phase but longer follow up and a comprehensive assessment of the role of demographic characteristics and disease severity is needed. The role of protective neutralising antibodies is emerging, with implications for therapeutics and vaccines. Large, cross-national cohort studies using appropriate statistical analysis and standardised serological assays and clinical classifications should be prioritised.

show abstract

“…As people who have had SARS-CoV-2 previously confirmed by PCR would probably be less likely to seek antibody testing than other people, we consider this lower estimate (84.7%) to be a more appropriate estimate of test sensitivity for a potential use case in which people were to choose to take the test to find out their own previous infection status. For an alternative potential use of population serosurveillance,34 the estimate of test sensitivity of 86.6% (83.2% to 89.4%), which derives from an analysis of all EDSAB-HOME stream A and B participants, irrespective of PCR positivity, may be more appropriate. Finally, we observed that AbC-19 test bands were often weak, a finding also reported in another laboratory based evaluation of AbC-19 16.…”

Section: Discussionmentioning

confidence: 99%

“…Most previous evaluations of LFIAs have used a “two gate” design, in which tests are performed on two groups of samples: PCR positives and pre-pandemic sera 24202122. This study design remains an important tool in evaluating accuracy, owing to the lack of a gold standard test, as discussed above.…”

Section: Discussionmentioning

confidence: 99%

“…Several lateral flow immunoassays (LFIAs)—small, pregnancy test format devices that can deliver testing rapidly and at scale—have recently become available that detect antibodies against SARS-CoV-2 proteins. These devices have two potential main uses: population serosurveillance and assessment of individual risk of developing immunity to coronavirus disease 2019 (covid-19) 345. The US Food and Drug Administration recently (24 September 2020) licensed an LFIA for office use (that is, in supervised environments), on the basis that it may predict immunity (https://www.fda.gov/media/139789/download); if this is validated, then it could result in widespread use of this class of devices.…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Accuracy of UK Rapid Test Consortium (UK-RTC) “AbC-19 Rapid Test” for detection of previous SARS-CoV-2 infection in key workers: test accuracy study

Mulchandani

¹

,

Jones

²

,

Taylor‐Phillips

³

et al. 2020

BMJ

View full text Add to dashboard Cite

Objective To assess the accuracy of the AbC-19 Rapid Test lateral flow immunoassay for the detection of previous severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) infection. Design Test accuracy study. Setting Laboratory based evaluation. Participants 2847 key workers (healthcare staff, fire and rescue officers, and police officers) in England in June 2020 (268 with a previous polymerase chain reaction (PCR) positive result (median 63 days previously), 2579 with unknown previous infection status); and 1995 pre-pandemic blood donors. Main outcome measures AbC-19 sensitivity and specificity, estimated using known negative (pre-pandemic) and known positive (PCR confirmed) samples as reference standards and secondly using the Roche Elecsys anti-nucleoprotein assay, a highly sensitive laboratory immunoassay, as a reference standard in samples from key workers. Results Test result bands were often weak, with positive/negative discordance by three trained laboratory staff for 3.9% of devices. Using consensus readings, for known positive and negative samples sensitivity was 92.5% (95% confidence interval 88.8% to 95.1%) and specificity was 97.9% (97.2% to 98.4%). Using an immunoassay reference standard, sensitivity was 94.2% (90.7% to 96.5%) among PCR confirmed cases but 84.7% (80.6% to 88.1%) among other people with antibodies. This is consistent with AbC-19 being more sensitive when antibody concentrations are higher, as people with PCR confirmation tended to have more severe disease whereas only 62% (218/354) of seropositive participants had had symptoms. If 1 million key workers were tested with AbC-19 and 10% had actually been previously infected, 84 700 true positive and 18 900 false positive results would be projected. The probability that a positive result was correct would be 81.7% (76.8% to 85.8%). Conclusions AbC-19 sensitivity was lower among unselected populations than among PCR confirmed cases of SARS-CoV-2, highlighting the scope for overestimation of assay performance in studies involving only PCR confirmed cases, owing to “spectrum bias.” Assuming that 10% of the tested population have had SARS-CoV-2 infection, around one in five key workers testing positive with AbC-19 would be false positives. Study registration ISRCTN 56609224.

show abstract

“…The copyright holder for this this version posted September 27, 2020. ; https://doi.org/10.1101/2020.09.25.20183459 doi: medRxiv preprint sensitivity (21% to 92%), that was significantly inferior to ELISAs performed on venous blood (Flower et al, 2020). Studies have shown high sensitivity of ELISAs for the detection of SARS-CoV-2 antibodies in venous blood (Adams et al, 2020;Lisboa Bastos et al, 2020;Staines et al, 2020).…”

Section: Introductionmentioning

confidence: 99%

Self-sampling of capillary blood for serological testing of SARS-CoV-2 by COVID-19 IgG ELISA

Brown

¹

,

Byrne

²

,

Fraser

³

et al. 2020

Preprint

View full text Add to dashboard Cite

Serological testing is emerging as a powerful tool to progress our understanding of COVID-19 exposure, transmission and immune response. Large-scale testing is limited by the need for in-person blood collection by staff trained in venepuncture. Capillary blood self-sampling and postage to laboratories for analysis could provide a reliable alternative. Two-hundred and nine matched venous and capillary blood samples were obtained from thirty nine participants and analysed using a COVID-19 IgG ELISA to detect antibodies against SARS-CoV-2. Thirty seven out of thirty eight participants were able to self-collect an adequate sample of capillary blood (≥50 μl). Using plasma from venous blood collected in lithium heparin as the reference standard, matched capillary blood samples, collected in lithium heparin-treated tubes and on filter paper as dried blood spots, achieved a Cohen′s kappa coefficient of >0.88 (near-perfect agreement). Storage of capillary blood at room temperature for up to 7 days post sampling did not affect concordance. Our results indicate that capillary blood self-sampling is a reliable and feasible alternative to venepuncture for serological assessment in COVID-19.

show abstract

Clinical and laboratory evaluation of SARS-CoV-2 lateral flow assays for use in a national COVID-19 seroprevalence survey

Cited by 136 publications

References 24 publications

Antibody response to SARS-CoV-2 infection in humans: a systematic review

Antibody response to SARS-CoV-2 infection in humans: a systematic review

Accuracy of UK Rapid Test Consortium (UK-RTC) “AbC-19 Rapid Test” for detection of previous SARS-CoV-2 infection in key workers: test accuracy study

Self-sampling of capillary blood for serological testing of SARS-CoV-2 by COVID-19 IgG ELISA

Contact Info

Product

Resources

About