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DETECTION OF EUBACTERIA IN INTERSTITIAL CYSTITIS BY 16S rDNA AMPLIFICATION
Authors:Dianne M. Heritz  Jean-Michel Y. Lacroix  Sukhsatej D. Batra  Keith A. Jarvi  B. Beheshti  Marc W. Mittelman
Affiliation:

aFrom the Women's College Hospital, Centre for Infection and Biomaterials Research, Mount Sinai Hospital, Departments of Surgery, University of Toronto, Toronto, Ontario, Canada.

bAccepted for publication June 6, 1997.

c(Heritz) Requests for reprints: The Urology Clinic, 100 Fourth Avenue, St. Catharines, Ontario, Canada, L2S 3P3.

dSupported by grants from the Physicians' Services Incorporated Foundation, North York, Ontario, Bayer, Canada, and the Natural Science and Engineering Research Council of Canada.

Abstract:

Objective

To determine what role non-culturable microorganisms play in the etiology of interstitial cystitis (IC).

Materials and Methods

Thirty patients fulfilling NIH criteria for the diagnosis of interstitial cystitis and sixteen control patients with culture negative urine gave written informed consent and underwent bladder biopsy. Polymerase chain reaction (PCR) using two sets of universal primers for bacterial 16S rDNA was performed on urine from the cystoscope and on a cold cup bladder biopsy specimen. Of the PCR positive bladder biopsies, three patients with interstitial cystitis and three controls were randomly selected and cloned. Ten clones from each were sequenced and putative taxonomic assignments made.

Results

12/26 (46%) IC and 5/12 (42%) control urine specimens and 16/30 (53%) and 9/15 (60%) bladder biopsies were PCR positive, respectively. The bacterial populations in the two patient groups tested appeared to be different based upon analysis of the 16S rRNA sequences.

Conclusions

Both IC and control patients had non-culturable bacteria in their bladders. A random sampling of the two populations revealed that the bacterial populations are different, suggesting a possible link between one or more bacterial species and IC.
Keywords:
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