Laboratory strategies for efficient handling of paraffin-embedded tissues for molecular detection of clonality in non-Hodgkin lymphomas

被引:19
|
作者
Stefanoff, CG
Hassan, R
Gonzalez, AC
Andrade, LAB
Tabak, DG
Romano, S
Zalcberg, IR
机构
[1] INCa CEMO, Inst Nacl Canc, BR-20230130 Rio De Janeiro, Brazil
[2] Univ Fed Fluminense, Inst Biol, Niteroi, RJ, Brazil
[3] Fed Univ Rio De Janeiro, Dept Genet, Rio De Janeiro, Brazil
[4] Inst Nacl Canc, Serv Patol, Rio De Janeiro, Brazil
关键词
paraffin-embedded tissue; DNA extraction; clonality assays PCR; non-Hodgkin lymphomas;
D O I
10.1097/00019606-200306000-00003
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
We herein present a technical strategy to optimize DNA isolation from paraffin-embedded tissue (PET). This includes the choice of adequate buffers for proteinase K digestion and multiplex PCR amplifications for assessing the appropriateness of DNA extracts for subsequent PCR assays for detecting clonality. We found that the association of proteinase K digestion in nonionic buffer and subsequent extract dilutions accounted for 79% of successful amplifications. A final efficiency of 88% was achieved by additional organic extractions and/or re-extractions. Comparisons were carried out with control DNA extracts from fresh samples to assess the efficiency of each clonality assay. Immunoglobulin CDRIII rearranged region amplification was more efficient for pregerminal center B-cell lymphomas in contrast to CDRII rearrangement detection, which Was more effective for germinal and postgerminal lymphomas. T-cell clonality detection by TCRgamma PCR was less efficient in PET samples than in fresh tissues showing that DNA integrity is more critical for TCR than for IGH amplification. Two inconclusive cases without phenotypic markers and two other atypical lymphoproliferations masked by reactive T cells were diagnosed as plasmabiastic lymphomas and as monoclonal B-proliferations, respectively, due to IGH rearrangements.
引用
收藏
页码:79 / 87
页数:9
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