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a Department of
Histopathology, Southampton General Hospital, Southampton, UK, b Histocompatibility
and Immunogenetics Laboratory, Southampton General Hospital,
Southampton, UK, c Department of Cellular Pathology, John Radcliffe
Hospital, Oxford, UK
Correspondence to: Dr A C Bateman, Department of Histopathology, Level E, South Block, Southampton General Hospital, Tremona Road, Southampton SO16 6YD, UK.
Accepted for publication 17 February 1999
BACKGROUND
Mislabelling or
contamination of surgical specimens may lead to diagnostic inaccuracy,
particularly within gastrointestinal pathology when multiple small
mucosal biopsy specimens are commonly taken, and where a tiny fragment
of foreign tissue may be indistinguishable from true biopsy material
using histological assessment alone.
AIMS
To assess the utility of
polymerase chain reaction (PCR) based human leucocyte antigen (HLA)
genotyping techniques for the investigation of potentially mislabelled
or contaminated gastrointestinal biopsy specimens.
PATIENTS
Ten cases (28 samples) in which mislabelling or contamination was suspected,
comprising four upper gastrointestinal tract biopsies and six
colonoscopic biopsy series.
METHODS
Direct and nested
PCR-sequence specific primer (SSP) based HLA class II genotyping was
performed on DNA extracted from formalin fixed and paraffin wax
embedded tissue (23 samples) or peripheral blood leucocytes (five samples).
RESULTS
A full HLA-DRB1 genotype
was determined in all 28 samples. In seven cases the HLA-DRB1 genotype
of the putative contaminant was different to that of the corresponding
reference tissue, confirming different individual origins for the
contaminant and reference material. In one case the contaminant tissue
was shown to possess the same HLA-DRB1 alleles as a second patient
(probable source). In the remaining three cases the same HLA-DRB1
alleles were detected within the potential contaminant and reference tissues.
CONCLUSIONS
PCR based HLA class II
genotyping is a valuable tool for investigating potential contamination
or mislabelling within gastrointestinal biopsy specimens and this
report has confirmed contamination in seven of ten cases studied.
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