Optimization and Validation of a Multiplexed Luminex Assay To Quantify Antibodies to Neutralizing Epitopes on Human Papillomaviruses 6, 11, 16, and 18

Author:

Dias Dennis1234,Van Doren Jeff1234,Schlottmann Sonela1234,Kelly Sheri1234,Puchalski Derek1234,Ruiz Wanda1234,Boerckel Patricia1234,Kessler Joseph1234,Antonello Joseph M.1234,Green Tina1234,Brown Martha1234,Smith Judith1234,Chirmule Narendra1234,Barr Eliav1234,Jansen Kathrin U.1234,Esser Mark T.1234

Affiliation:

1. Vaccine and Biologics Research, Merck Research Laboratories, 466 Devon Park Dr., Wayne, Pennsylvania 19087-8630

2. Vaccine Biometrics Research

3. Vaccine and Biologics Research, Merck Research Laboratories, West Point, Pennsylvania 19486

4. Vaccine and Biologics Clinical Research, Merck Research Laboratories, Blue Bell, Pennsylvania 19422

Abstract

ABSTRACT A human papillomavirus (HPV) multiplexed competitive Luminex immunoassay first described by Opalka et al. (D. Opalka, C. E. Lachman, S. A. MacMullen, K. U. Jansen, J. F. Smith, N. Chirmule, and M. T. Esser, Clin. Diagn. Lab. Immunol. 10:108-115, 2003) was optimized and validated for use in epidemiology studies and vaccine clinical trials. Optimization increased both the analytical sensitivity and the clinical specificity of the assay to more effectively discriminate the low-titer antibody response of HPV-infected persons from noninfected individuals. The characteristics of the assay that were optimized included monoclonal antibody (MAb) specificity, scaling up the conjugation of virus-like particles (VLPs) to microspheres, VLP concentration, MAb concentration, sample matrix, sample dilution, incubation time, heat inactivation of sample sera, and detergent effects on assay buffer. The assay was automated by use of a TECAN Genesis Workstation, thus improving assay throughput, reproducibility, and operator safety. Following optimization, the assay was validated using several distinct serum panels from individuals determined to be at low and high risk for HPV infection. The validated assay was then used to determine the clinical serostatus cutoff. This high-throughput assay has proven useful for performing epidemiology studies and evaluating the efficacy of prophylactic HPV vaccines.

Publisher

American Society for Microbiology

Subject

Microbiology (medical),Clinical Biochemistry,Immunology,Immunology and Allergy

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