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Identification of T-cell receptor expression in EBV-positive neoplastic cells in extranodal NK/T-cell lymphoma, nasal-type, and comparison with T-cell receptor gene rearrangement by BIOMED-2 assay

机译:EBV阳性肿瘤细胞中T细胞受体表达在外侧NK / T细胞淋巴瘤,鼻型的鉴定及与生物密合 - 2测定的T细胞受体基因重排的比较

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摘要

The cellular lineage of extranodal NK/T-cell lymphoma, nasal-type (ENKTL), is determined by expression of T-cell receptor (TR) orTRgene rearrangement. In ENKTL, from TR immunohistochemistry, it may often be difficult to decide whether TR-positive cells are tumor cells or not, especially when TR is expressed in a subset of tumor cells. To analyze TR expression pattern andTRrearrangement in T-lineage ENKTL, we performed double immunofluorescence staining for Epstein-Barr virus–encoded small RNAs (EBER)/T-cell receptor (TCR)βF1 and CD56/TCRβF1 in 12 cases of ENKTL that showed TCRβF1 expression in immunohistochemistry.TRgene rearrangement was analyzed using a commercial BIOMED-2 multiplex polymerase chain reaction system. Immunohistochemistry showed that all 12 cases expressed TCRβF1 in a wide range of infiltrating cells from 100% to <1%. Two of them expressed both TCRβF1 and TCR cγM1. EBER/TCR-βF1–positivity was confirmed in 10 cases by double staining. One case failed to show EBER/TCR-βF1–positive cells but showed a CD56/TCRβF1–positive result. Among 12 cases, 5 had poor-quality DNA, 3 of them showed no polymerase chain reaction product, and 2 cases showed nonspecific peak of low height. Five of 7 cases with good DNA quality demonstrated monoclonalTRgene rearrangement. Based onTRexpression andTRgene rearrangement, 10 of 12 cases of ENKTL were decided as a T-lineage tumor. In conclusion, because of common TR silence and poor DNA quality, consideration of both immunohistochemistry andTRgene rearrangement is necessary to determine the lineage of ENKTL.
机译:通过表达T细胞受体(Tr)甘油重新排列来确定外骨NK / T细胞淋巴瘤的细胞谱系,鼻型(ENKT1)。在eNKTL中,从TR免疫组织化学,通常难以确定TR阳性细胞是否是肿瘤细胞,特别是当TR在肿瘤细胞的子集中表达时。为了分析T轴线ENKT1中的TR表达模式和特征,我们对显示TCRβF1的ENKT1的12例进行了对Epstein-BART病毒编码的小RNA(EBER)/ T细胞受体(TCR)βF1和CD56 /TCRβF1的双重免疫荧光染色免疫组织化学中的表达。使用商业生物学-2多重聚合酶链式反应系统分析了乙烯重排。免疫组织化学表明,所有12例都表达了渗透细胞范围内的TCRβF1,从100%到<1%。其中两个表达了TCRβF1和TCRCγM1。通过双染色在10例中确认EBER / TCR-βF1阳性。一种情况未能显示EBER / TCR-βF1阳性细胞,但显示CD56 /TCRβF1阳性结果。在12例患者中,5种质量差的DNA,其中3个显示出没有聚合酶链反应产物,2例显示低高度的非特异性峰。 7例良好的DNA质量中的五种患者展示了单克诺术后重排。基于对易患的andTrgene重新排列,12例ENKTL的10例被认为是T族肿瘤。总之,由于常见的TR沉默和差的DNA质量,考虑免疫组织化学andtrgene重排是确定enktl的谱系必需的。

著录项

  • 来源
    《Human Pathology》 |2018年第2018期|共8页
  • 作者单位

    Department of Pathology and Translational Genomics Samsung Medical Center Sungkyunkwan University;

    Department of Pathology and Translational Genomics Samsung Medical Center Sungkyunkwan University;

    Department of Pathology and Translational Genomics Samsung Medical Center Sungkyunkwan University;

    Section of Hematology-Oncology Department of Internal Medicine Samsung Medical Center;

    Section of Hematology-Oncology Department of Internal Medicine Samsung Medical Center;

    Department of Pathology and Translational Genomics Samsung Medical Center Sungkyunkwan University;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 病理学;
  • 关键词

    Extranodal; NK/T; Lymphoma; T cell receptor; Expression; Gene rearrangement;

    机译:外结;NK / T;淋巴瘤;T细胞受体;表达;基因重排;

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