Campylobacter species, especially Campylobacter jejuni and Campylobacter coli, are a major cause of human bacterial enteritis. Current detection in stools is done essentially by culture on selective and nonselective media with filtration. These methods were compared to 2 molecular biology methods, an in-house real-time PCR and a multiplex PCR named Seeplex Diarrhea ACE Detection, and 3 immunoenzymatic methods, Premier Campy, RidaScreen Campylobacter, and ImmunoCard Stat!Campy. Out of 242 stool specimens tested, 23 (9.5%) fulfilled the positivity criteria, i.e., they were positive by one or both culture methods or, in case of a negative culture, by a positive molecular method and a positive immunoenzymatic method. The striking feature of this study is the low sensitivity of culture, in the range of 60%, in contrast to immunoenzymatic and molecular tests.The incidence of Campylobacter-associated food poisoning has gradually increased, and the organism is now considered to be the leading cause of bacterial gastroenteritis worldwide (4). These infections can also lead to extraintestinal diseases and severe long-term complications (9). Campylobacter jejuni and Campylobacter coli are the most frequently isolated species in this context and in our experience account for 80% and 16%, respectively, of all the isolates received in our laboratory every year (2a). Campylobacter species are bacteria with a special culture requirement, i.e., a microaerobic environment. During stool processing, the bacteria may have long contact with a normal atmosphere, and in addition, the progressive decrease in oxygen tension when gas-generating kits are used may not favor adequate growth. Furthermore, selective media are commonly used, and the antibiotics incorporated may inhibit certain Campylobacter strains. Anecdotal data have shown that spiral or curved bacteria are sometimes observed on stool smears while Campylobacter growth does not occur. In a recent study, DNA sequences of the Campylobacter genome were detected by a metagenomic analysis, while the standard culture methods were negative (5). In a pilot study using real-time PCR as a diagnostic tool, we also detected more campylobacters than with culture, but without being able to confirm that true positives were detected, since, at that time, we did not use multiple detection methods to establish positivity when culture was negative. Some immunoenzymatic tests have already been commercialized for several years, such as the ProSpecT Campylobacter Microplate Assay (Remel) (8) and the RidaScreen Campylobacter (R-Biopharm, Darmstadt, Germany) evaluated in our study. In this study, we took advantage of the availability of several kits to compare Campylobacter detection by molecular methods (2 PCRs) and by 3 immunoenzymatic methods to the standard culture methods.
MATERIALS AND METHODS
Materials.From 15 June to 30 October 2009, every stool specimen obtained from a symptomatic patient, i.e., a patient with a gastrointestinal illness, who was hospitalized for less than 48 h at Pellegrin H...
