BMC Infectious Diseases (Apr 2011)

Sequential multiplex PCR assay for determining capsular serotypes of colonizing <it>S. pneumoniae</it>

  • Melderen Laurence Van,
  • Verhaegen Jan,
  • Vandeven Jozef,
  • Drèze Pierre-Alexandre,
  • Jourdain Sarah,
  • Smeesters Pierre R

DOI
https://doi.org/10.1186/1471-2334-11-100
Journal volume & issue
Vol. 11, no. 1
p. 100

Abstract

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Abstract Background Asymptomatic nasopharyngeal carriage represents an important biological marker for monitoring pneumococcal serotype distribution and evaluating vaccine effects. Serotype determination by conventional method (Quellung reaction) is technically and financially challenging. On the contrary, PCR-based serotyping represents a simple, economic and promising alternative method. Method We designed a novel multiplex PCR assay for specific detection of the 30 classical colonizing S. pneumoniae serogroups/types. This multiplex assay is composed of 7 consecutive PCR reactions and was validated on a large and recent collection of Streptococcus pneumoniae isolated during a prospective study conducted in Belgium at the time of PCV7 adoption. Results The multiplex PCR assay allowed the typing of more than 94% of the isolates of a collection of pneumococci isolated from Belgian preschool attendees (n = 332). Seventy-five percent of the isolates were typed after 3 subsequent PCR reactions. Results were in agreement with the Quellung identification. Conclusion Our novel multiplex assay is an accurate and reliable method which can be used in place of the conventional method for S. pneumoniae carriage studies.