All swabs should be processed; however, to assist with interpreting the results, investigators should record whether the procedure was acceptable or suboptimal. Recording if secretions are present on the swab [18] and whether the swab was potentially contaminated (e.g. touched by the investigator or dropped on the ground) may also be helpful in interpretation. Because NP specimen collection (by swab or by wash) requires training, demands adherence
to the methodology, and is unpleasant for the study subject, and because sometimes even nasal swabs are not well tolerated, alternate Panobinostat research buy methods have been assessed. Leach et al. [19] found that in an Australian population with a high pneumococcal burden, nose blowing into a paper tissue, followed by swabbing and culture of the material on the tissue, was an effective alternative
to nasal swabbing when nasal secretions were present. The sensitivity of detecting pneumococcus from nose blowing samples (compared with nasal swabs, and when secretions were visible at the time of sampling) was 97% in Aboriginal children aged 3–7 years and 94% in children aged less than 4 years who were attending urban child care centers. For children without visible secretions, direct NP or nasal sampling was required [19]. Recently, Sorafenib chemical structure Van den Bergh et al. [14] found that the proportion of pneumococcal-positive cultures was similar when sampling secretions from a tissue (tissue swab 65%, whole tissue 74%), or taking NP and nasal swabs (both 64%) in 66 Dutch children aged 0–4 years with rhinorrhea. Data relating to detection of H. influenzae, M. catarrhalis, S. aureus and respiratory viruses by various sampling methods are described in the Supplementary Material (including Supplementary Table 3). We recommend the NP swab approach for collection of the sample. NP aspirates or washes are also acceptable methods of specimen
collection as they have sensitivity for pneumococcal detection equal to, or greater than, that of NP swabs, but may GBA3 be less tolerated by participants. In the event that NP sampling cannot be implemented, nasal swabs or swabbing visible secretions from nose blowing into a tissue are better than collecting no specimens. However, any deviation from the recommended NP swab should be clearly reported to allow accurate comparisons across studies. All data presented are from studies using culture to detect pneumococci. Specimen collection comparison studies should be undertaken using molecular methods for pneumococcal detection. Direct comparisons of NP and nasal sampling methods in healthy children are also needed. A single NP swab is unlikely to represent the colonizing bacteria of the upper respiratory tract with complete sensitivity, as these bacteria may not reside uniformly across the mucosal surface, and there is inherent variability in the mucosal surfaces touched by each sample swab.