Literature DB >> 17620388

Analysis of T-cell clonality using laser capture microdissection and high-resolution microcapillary electrophoresis.

Evgeny Yakirevich1, Cynthia L Jackson, Patricia A Meitner, Dolores MacKenzie, Rose Tavares, Leslie Robinson-Bostom, Ronald A DeLellis, Murray B Resnick.   

Abstract

Identification of clonal lymphocytic populations by polymerase chain reaction may be difficult in cases with scant cellular infiltrates or those with a heterogeneous population of cells. Here, we assessed the diagnostic utility of laser capture microdissection (LCM) and high-resolution microcapillary electrophoresis in the analysis of clonality of small biopsy specimens. Clonality was determined in 24 cases: five reactive tonsils, five reactive lymph nodes, six inflammatory skin lesions, and eight T-cell lymphomas. CD3-positive T lymphocytes were captured by LCM from paraffinized immunohistochemically stained sections. Genomic DNA was analyzed for T-cell receptor-gamma gene rearrangement by polymerase chain reaction followed by high-resolution microcapillary electrophoresis with the DNA 500 LabChip and the Agilent Bioanalyzer. In the reactive specimens, T-cell receptor-gamma polymerase chain reaction revealed monoclonal bands when 10 to 1000 cells were captured. This pattern changed to polyclonal when higher numbers of cells were microdissected (2000 to 10,000 cells). In contrast, lymphoma cells were consistently monoclonal whether low or high numbers were microdissected. Microcapillary electrophoresis coupled with LCM facilitated clonality analysis in equivocal cases. In two of eight lymphoma cases, LCM revealed diagnostic monoclonal bands, whereas routine T-cell receptor-gamma assessment of whole tissue sections with 10% polyacrylamide gel electrophoresis demonstrated only minor clonal bands. We conclude that clonality determined by LCM is cell number-dependent. Biopsy specimens containing low numbers of reactive polyclonal T cells may produce pseudomonoclonal bands and therefore should be interpreted with great caution.

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Year:  2007        PMID: 17620388      PMCID: PMC1975101          DOI: 10.2353/jmoldx.2007.070006

Source DB:  PubMed          Journal:  J Mol Diagn        ISSN: 1525-1578            Impact factor:   5.568


  43 in total

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2.  Effectiveness of capillary electrophoresis using fluorescent-labeled primers in detecting T-cell receptor gamma gene rearrangements.

Authors:  Timothy C Greiner; Ronald J Rubocki
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Review 3.  Microdissection techniques for molecular testing in surgical pathology.

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4.  Is clonality equivalent to malignancy: specifically, is immunoglobulin gene rearrangement diagnostic of malignant lymphoma?

Authors:  R D Collins
Journal:  Hum Pathol       Date:  1997-07       Impact factor: 3.466

5.  B-cell target DNA quantity is a critical factor in the interpretation of B-cell clonality by PCR.

Authors:  J M Taylor; D V Spagnolo; P H Kay
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6.  Clonal T-cell receptor gamma-chain gene rearrangement by PCR-based GeneScan analysis in advanced cutaneous T-cell lymphoma: a critical evaluation.

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9.  B-cell gene rearrangement in benign and malignant lymphoid proliferations of mucosa-associated lymphoid tissue and lymph nodes.

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4.  12-Chemokine gene signature identifies lymph node-like structures in melanoma: potential for patient selection for immunotherapy?

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5.  The role of molecular pathology in the diagnosis of cutaneous lymphomas.

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  5 in total

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