RT Journal Article SR Electronic(1) A1 Rajabally, Naayil A1 Kullin, Brian A1 Ebrahim, Kaleemuddeen A1 Brock, Tunehafo A1 Weintraub, Andrej A1 Whitelaw, Andrew A1 Bamford, Colleen A1 Watermeyer, Gillian A1 Thomson, Sandie A1 Abratt, Valerie A1 Reid, SharonYR 2016 T1 A comparison of Clostridium difficile diagnostic methods for identification of local strains in a South African centre JF Journal of Medical Microbiology, VO 65 IS 4 SP 320 OP 327 DO https://doi.org/10.1099/jmm.0.000231 PB Microbiology Society, SN 1473-5644, AB Accurate diagnosis of Clostridium difficile infection is essential for disease management. A clinical and molecular analysis of C. difficile isolated from symptomatic patients at Groote Schuur Hospital, South Africa, was conducted to establish the most suitable clinical test for the diagnosis and characterization of locally prevalent strains. C. difficile was detected in stool samples using enzyme-based immunoassays (EIA) and nucleic acid amplification methods, and their performance was compared with that of C. difficile isolation using direct selective culture combined with specific PCR to detect the C. difficile tpi gene, toxin A and B genes and binary toxin genes. Toxigenic isolates were characterized further by ribotyping. Selective culture isolated 32 C. difficile strains from 145 patients (22 %). Of these, the most prevalent (50 %) were of ribotype 017 (toxin A− B+) while 15.6 % were ribotype 001 (toxin A+B+). No ribotype 027 strains or binary toxin genes (cdtA and cdtB) were detected. The test sensitivities and specificities, respectively, of four commercial clinical diagnostic methods were as follows: ImmunoCard Toxins A & B (40 % and 99.1 %), VIDAS C. difficile Toxin A & B (50 % and 99.1 %), GenoType CDiff (86.7 % and 88.3 %) and Xpert C. difficile (90 % and 97.3 %). Ribotype 001 and 017 strains had a 100 % detection rate by Xpert C. difficile, 100 % and 93.3 % by GenoType CDiff, 75 % and 53.3 % by ImmunoCard and 75 % and 60 % by VIDAS, respectively. The overall poor performance of EIA suggests that a change to PCR-based testing would assist diagnosis and ensure reliable detection of locally prevalent C. difficile 017 strains., UL https://www.microbiologyresearch.org/content/journal/jmm/10.1099/jmm.0.000231