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Shin, Yoo, and Oh: Comparison of Two Enzyme Immunoassay for Detection of Clostridium difficile Toxin A and Toxin B
Original Article

Korean J Leg Med 2009;29(2):122-126.

Published online: 14 February 2009

DOI: https://doi.org/10.3343/kjlm.2009.29.2.122

Comparison of Two Enzyme Immunoassay for Detection of Clostridium difficile Toxin A and Toxin B

Bo-Moon Shin, M.D., Soo-Jin Yoo, M.D., Hye Jun Oh, M.T.

Department of Laboratory Medicine, Sanggye Paik Hospital, Inje University, Seoul, Korea

Corresponding author: Bo-Moon Shin, M.D. Department of Laboratory Medicine, Sanggye Paik Hospital, Inje University, 761-1 Sanggye 7-dong, Nowon-gu, Seoul 139-707, Korea Tel: +82-2-950-1227, Fax: +82-2-950-1224 E-mail: bmshin@unitel.co.kr

Received 11 November 20085 January 2009       Accepted 5 January 2009

Copyright © 2009 by the Korean Society for Legal Medicine

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Background

Enzyme immunoassay (EIA) capable of detecting both toxin A and toxin B is strongly recommended for the diagnosis of Clostridium difficile associated disease. Therefore, we evaluated two different EIAs for the detection of C. difficile toxin A/B.

Methods

For a total of 228 stool specimens we performed bacteriologic cultures for C. difficile and examined for toxin A and toxin B using enzyme linked fluorescent immunoassay (ELFA; VIDAS CDAB, Bio-Merieux sa, France) and ELISA (C.DIFFICILE TOX A/B II, TECHLAB, USA). We also performed PCR assays for toxin A and B genes in 117 C. difficile isolates that grew from the stool cultures and compared the results with those obtained with the two different EIAs.

Results

The concordance rate between ELFA and ELISA was 85.5% (195/228). Using the culture and PCR results as the standard, the sensitivity/specificity of the ELFA and ELISA were 65.0%/72.1% and 71.8%/70.3%, and for positive/negative predictive values were 78.4%/69.6% and 71.8%/70.3%, respectively (P value >0.05). No differences were observed between the results of ELFA and ELISA with toxin A toxin B+ strains of C. difficile.

Conclusions

The sensitivity of the ELISA was slightly higher than that of ELFA for toxin A and toxin B, but the specificity and positive predictive value of the ELFA were rather higher than those of the ELISA, although no statistical differences were observed. A bacteriologic culture and PCR assay for toxin genes are recommended in case the both EIAs are negative.

Keywords: Clostridium difficile, Toxin A, Toxin B, Enzyme immunoassay, PCR

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Table 1.
Comparison of toxin A and B enzyme immunoassay results
  ELFA (VIDAS) Total
(+) equivocal (–)
ELISA (+) 96 5 16 117
(TECHLAB) (–) 1 11 99 111
Total 97 16 115 228

Abbreviation: ELFA, enzyme linked fluorescent assay.

Table 2.
Comparison of ELFA (VIDAS) and ELISA (TECHLAB) tests with C. difficile culture and PCR assay detecting both toxin A and B
  Culture positive (N=155) Culture negative (N=73) Total
PCR positive PCR negative
ELFA        
 + 76 (65.0%) 4 (10.5%) 17 (23.3%) 97 (42.6%)
 Equivocal 6 (5.1%) 3 (7.9%) 7 (9.6%) 16 (7.0%)
 - 35 (29.9%) 31 (81.6%) 49 (67.1%) 115 (50.4%)
ELISA        
 + 84 (71.8%) 7 (18.4%) 26 (35.6%) 11 7 (51.3%)
 - 33 (28.2%) 31 (81.6%) 47 (64.4%) 111 (48.7%)
Total 117 (100%) 38 (100%) 73 (100%) 228 (100%)

C. difficile toxin A and/or toxin B gene positive strains

Abbreviation: ELFA, enzyme linked fluorescent assay.

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