Silver-enhanced in situ hybridization for detection of polyomavirus DNA in patients with BK virus nephropathy

BK virus nephropathy is not an infrequent complication of renal transplantation associated with high rates of graft loss. Although antibodies against SV40 antigen detect different viruses of the polyomavirus family, immunohistochemistry is widely used to confirm the diagnosis of BK virus nephropathy...

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Published inDiagnostic molecular pathology Vol. 20; no. 2; p. 105
Main Authors Fritzsche, Florian R, Pianca, Silvio, Gaspert, Ariana, Varga, Zsuzsanna, Wang, Lin, Farrell, Michael P, Chen, Xiao-Bo, Hirsch, Hans H, Springer, Erik, Fehr, Thomas, Myles, Jonathan, Tubbs, Raymond, Moch, Holger
Format Journal Article
LanguageEnglish
Published United States 01.06.2011
Subjects
Adolescent
Adult
Aged
Automation - methods
BK Virus - genetics
BK Virus - isolation & purification
DNA, Viral - genetics
DNA, Viral - isolation & purification
Female
Humans
In Situ Hybridization - methods
Kidney Diseases - diagnosis
Kidney Diseases - virology
Kidney Transplantation - adverse effects
Male
Middle Aged
Polyomavirus Infections - diagnosis
Polyomavirus Infections - virology
Sensitivity and Specificity
Silver - metabolism
Staining and Labeling - methods
Young Adult
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Summary:BK virus nephropathy is not an infrequent complication of renal transplantation associated with high rates of graft loss. Although antibodies against SV40 antigen detect different viruses of the polyomavirus family, immunohistochemistry is widely used to confirm the diagnosis of BK virus nephropathy in renal biopsies. Here we aimed to validate the novel silver-enhanced in situ hybridization (SISH) technique for the automated detection of BK virus in renal transplant biopsies. Two different patient cohorts were included. Twenty-nine consecutive patients suspicious for BK virus infection were investigated by SISH and chromogenic in situ hybridization. An additional 26 renal biopsies positive by SV40 immunohistochemistry from 19 patients were analyzed by SISH. Polyomavirus DNA serum levels, as determined by nested PCR analysis, were available for all of these patients. The presence of BK virus DNA in renal tubular cells was identified in 5 of the suspicious cases by both, SISH and chromogenic in situ hybridization . One additional patient was only positive in the SISH. In the second cohort, SISH was positive in all SV40 positive biopsies, but SISH signals were less extensive than SV40 immunohistochemistry. Our results show that the BK virus SISH is an ancillary tool for the detection of polyomavirus DNA in renal biopsies using bright-field microscopy. However, its diagnostic value in comparison with standard immunohistochemistry seems to be limited.
ISSN:1533-4066
DOI:10.1097/PDM.0b013e3182015074