Evaluation of a Novel Microarray Immunoblot Assay for Detection of IgM- and IgG-Class Antibodies to Borrelia burgdorferi

Theel, Elitza S.; Sorenson, Marisa; Granger, Dane

doi:10.1128/jcm.00992-18

Cited by 9 publications

(9 citation statements)

References 22 publications

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“…In conclusion, several investigations using the multi-antigen approach to improve serologic testing for Lyme disease have been reported underscoring the rationalization for adding antigens for new test algorithms (14–18). A commercial assay would likely employ multiplex testing technology to enhance sensitivity over ELISA formats and provide a platform to screen dozens of antigens (11, 19, 20). These studies and ours represent pilot versions of algorithms for new tests and warrant validation with higher numbers of prospectively and retrospectively collected patient samples.…”

Section: Discussionmentioning

confidence: 99%

Evaluation of Patient IgM and IgG Reactivity Against Multiple Antigens for Improvement of Serodiagnostic Testing for Early Lyme Disease

Brandt

Horiuchi

Biggerstaff

et al. 2019

Front. Public Health

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Serologic testing is the standard for laboratory diagnosis and confirmation of Lyme disease. Serodiagnostic assays to detect antibodies against Borrelia burgdorferi, the agent of Lyme borreliosis, are used for detection of infection. However, serologic testing within the first month of infection is less sensitive as patients' antibody responses continue to develop. Previously, we screened several B. burgdorferi in vivo expressed antigens for candidates that elicit early antibody responses in patients with Stage 1 and 2 Lyme disease. We evaluated patient IgM seroreactivity against 6 antigens and found an increase in sensitivity without compromising specificity when compared to current IgM second-tier immunoblot scoring. In this study, we continued the evaluation using a multi-antigen panel to measure IgM plus IgG seroreactivity in these early Lyme disease patients' serum samples. Using two statistical methods for calculating positivity cutoff values, sensitivity was 70 and 84–87%, for early acute and early convalescent Lyme disease patients, respectively. Specificity was 98–100% for healthy non-endemic control patients, and 96–100% for healthy endemic controls depending on the statistical analysis. We conclude that improved serologic testing for early Lyme disease may be achieved by the addition of multiple borrelial antigens that elicit IgM and IgG antibodies early in infection.

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Section: Discussionmentioning

confidence: 99%

Evaluation of Patient IgM and IgG Reactivity Against Multiple Antigens for Improvement of Serodiagnostic Testing for Early Lyme Disease

Brandt

Horiuchi

Biggerstaff

et al. 2019

Front. Public Health

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“…In neuroborreliosis from two European countries, the IgG seroreactivity of VlsE alone surpassed that of other antigens commonly used (p100, p58, p39, OspA, OspC, and p18) compared to control patients (Dessau et al, 2015). IB have been recently miniaturized in a microarray format with probable equivalent performances to other commercial immunoblots (Theel et al, 2018). Given the diversity of genospecies involved in Lyme borreliosis in Europe compared to the US, almost all of the available IB kits use combinations of recombinant antigens from strains belonging to different species, generally the three main European pathogenic species (B. afzelii, B. garinii, B. burgdorferi ss) possibly associated with B. bavariensis and B. spielmanii, also responsible for some cases of Lyme borreliosis.…”

Section: Second Step Serology Testsmentioning

confidence: 99%

Immunoserological Diagnosis of Human Borrelioses: Current Knowledge and Perspectives

Talagrand-Reboul

Raffetin

Zachary

et al. 2020

Front. Cell. Infect. Microbiol.

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“…The STTT has been a useful diagnostic tool since its standardization by the Centers for Disease Control (CDC) in 1995 [13], but critical limitations have become increasingly apparent [16,17]. These include low sensitivity and low specificity for early disease [18,19], inability to monitor treatment progress or diagnose re-infection [20], inconsistencies across tests [21][22][23], and subjective interpretation of Western blot results [18,24]. Experts agree that new strategies for diagnosing LD are necessary to address these concerns, pointing to modified two-tier algorithms using only ELISAs [23,[25][26][27], as well as novel assays in various stages of development [28][29][30].…”

Section: Introductionmentioning

confidence: 99%

“…In this study, we systematically optimized and validated the GC-FP biochip for detection of specific serum antibodies in patients with untreated LD, patients treated for LD with antibiotics, and various negative controls using well characterized serum samples [22,43]. We hypothesized that GC-FP analysis could be used to effectively: 1) screen for antibody targets relevant to various stages of LD, and 2) allow us to develop a new algorithm for diagnosing disease status that is more sensitive, specific, and informative than the STTT.…”

Section: Introductionmentioning

confidence: 99%

A fluorescent plasmonic biochip assay for multiplex screening of diagnostic serum antibody targets in human Lyme disease

et al. 2020

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Lyme disease (LD) diagnosis using the current two-tier algorithm is constrained by low sensitivity for early-stage infection and ambiguity in determining treatment response. We recently developed a protein microarray biochip that measures diagnostic serum antibody targets using grating-coupled fluorescent plasmonics (GC-FP) technology. This strategy requires microliters of blood serum to enable multiplexed biomarker screening on a compact surface and generates quantitative results that can be further processed for diagnostic scoring. The GC-FP biochip was used to detect serum antibodies in patients with active and convalescent LD, as well as various negative controls. We hypothesized that the quantitative, high-sensitivity attributes of the GC-FP approach permit: 1) screening of antibody targets predictive for LD status, and 2) development a diagnostic algorithm that is more sensitive, specific, and informative than the standard ELISA and Western blot assays. Notably, our findings led to a diagnostic algorithm that may be more sensitive than the current standard for detecting early LD, while maintaining 100% specificity. We further show that analysis of relative antibody levels to predict disease status, such as in acute and convalescent stages of infection, is possible with a highly sensitive and quantitative platform like GC-FP. The results from this study add to the urgent conversation regarding better diagnostic strategies and more effective treatment for patients affected by tick-borne disease.

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Evaluation of a Novel Microarray Immunoblot Assay for Detection of IgM- and IgG-Class Antibodies to Borrelia burgdorferi

Cited by 9 publications

References 22 publications

Evaluation of Patient IgM and IgG Reactivity Against Multiple Antigens for Improvement of Serodiagnostic Testing for Early Lyme Disease

Evaluation of Patient IgM and IgG Reactivity Against Multiple Antigens for Improvement of Serodiagnostic Testing for Early Lyme Disease

Immunoserological Diagnosis of Human Borrelioses: Current Knowledge and Perspectives

A fluorescent plasmonic biochip assay for multiplex screening of diagnostic serum antibody targets in human Lyme disease

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