Evaluation of a Novel Multiplex High-Definition PCR Assay for Detection of Tick-Borne Pathogens in Whole-Blood Specimens

Blake W Buchan; Dean A Jobe; Michael Mashock; Derek Gerstbrein; Matthew L Faron; Nathan A Ledeboer; Steven M Callister

doi:10.1128/JCM.00513-19

Evaluation of a Novel Multiplex High-Definition PCR Assay for Detection of Tick-Borne Pathogens in Whole-Blood Specimens

J Clin Microbiol. 2019 Oct 23;57(11):e00513-19. doi: 10.1128/JCM.00513-19. Print 2019 Nov.

Authors

Blake W Buchan¹, Dean A Jobe², Michael Mashock³, Derek Gerstbrein³, Matthew L Faron³, Nathan A Ledeboer³, Steven M Callister²

Affiliations

¹ Department of Pathology, The Medical College of Wisconsin, Milwaukee, Wisconsin, USA bbuchan@mcw.edu.
² Microbiology Research and Molecular Diagnostics Laboratories, Gundersen Medical Foundation, La Crosse, Wisconsin, USA.
³ Department of Pathology, The Medical College of Wisconsin, Milwaukee, Wisconsin, USA.

Abstract

The prevalence of tick-borne infections has been steadily increasing in both number and geographic distribution in the United States and abroad. This increase, in conjunction with the continued recognition of novel pathogens transmitted by ticks, has made accurate diagnosis of these infections challenging. Mainstay serologic tests are insensitive during the acute phase of infection and are often cross-reactive with similar pathogenic and nonpathogenic organisms. Further, they are unable to reliably differentiate active versus past infection which can lead to misdiagnosis and incorrect understanding of the epidemiology and incidence of specific tick-borne pathogens. We evaluated a novel multiplexed high-definition PCR (HDPCR) Tickborne Panel (TBP) assay (ChromaCode, Carlsbad, CA) for the detection of nine tick-borne pathogens or groups associated with human illness. The HDPCR technology enables multiplex identification of multiple targets in a single fluorometric channel based on fluorescent signal modulation using a limiting probe design. A collection of 530 whole-blood specimens collected from patients being evaluated for tick-borne infections, in addition to a panel of 93 simulated specimens, were used to challenge the HDPCR TBP. The results were compared to a clinically validated traditional multiplexed PCR test with additional sequence analysis and clinical history collected to aid in resolving discrepancies. Among clinical specimens the TBP demonstrated 100% sensitivity for the identification of Anaplasma phagocytophilum, Borrelia miyamotoi, Borrelia mayonii, and Rickettsia rickettsii The sensitivity for identification of B. burgdorferi was 44.4% compared to a composite gold standard. Among simulated specimens containing single or multiple targets present at 10³ to 10⁵ copies/PCR, the sensitivity of TBP was 100% for all targets, with a combined specificity of 99.5%. Of note, an increased rate of false-positive results was observed among simulated specimens that contained multiple targets. Based on these data, we find the HDPCR TBP to be a useful adjunct for the diagnosis of tick-borne infections in patients with suspected tick-borne illness.

Keywords: high-definition PCR; tick-borne pathogens.

Publication types

Evaluation Study

MeSH terms

Bacteria / isolation & purification*
Bacteria / pathogenicity
Bacterial Proteins / genetics
False Positive Reactions
Fluorescence
Fluorescent Dyes
Humans
Multiplex Polymerase Chain Reaction / methods*
Sensitivity and Specificity
Tick-Borne Diseases / blood*
Tick-Borne Diseases / diagnosis*

Substances

Bacterial Proteins
Fluorescent Dyes