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抗T细胞受体Vβ抗体未能始终如一地识别蕈样肉芽肿综合征中的恶性T细胞克隆。

Failure of anti-T-cell receptor V beta antibodies to consistently identify a malignant T-cell clone in Sézary syndrome.

作者信息

Bigler R D, Boselli C M, Foley B, Vonderheid E C

机构信息

Department of Medicine, Medical College of Pennsylvania, Philadelphia, USA.

出版信息

Am J Pathol. 1996 Nov;149(5):1477-83.

Abstract

Monoclonal antibodies (MAbs) reacting with the human T cell receptor (TCR) V beta or V alpha region have been shown to be almost as specific as a private idiotypic MAb in identifying T cell clones. When available, V beta-specific MAbs offer the ease of immunofluorescence analysis to identify and quantitate expanded malignant or nonmalignant T cell populations without requiring polymerase chain reaction (PCR) technology to evaluate expression of V beta gene families. The V beta expression of peripheral blood lymphocytes from twenty-three consecutive patients with Sézary syndrome has been analyzed by reverse transcriptase (RT)-PCR. Ten patients had malignant T cell clones that expressed a TCR V beta corresponding to a commercially available anti-V beta antibody. Immunofluorescence staining with anti-V beta MAbs showed a direct correlation with RT-PCR results in seven of ten patients. No false positive reactivity was noted on immunofluorescence staining with any MAb. Cells from three patients, however, did not react with the corresponding anti-V beta MAb. These three cases expressed a TCR V beta from gene families containing a single member, ie, V beta 14, V beta 18, and V beta 20, yet MAbs reported to be specific for these regions failed to react with the T cell clone from these patients. Sequencing of the PCR product in these cases confirmed the RT-PCR results. Cells from two patients expressed a TCR using V beta 5.1-D beta 1.1 genes with different J-C segments. One patient's cells reacted with an anti-V beta 5.1 MAb (LC4) whereas the other patient's cells bound one-tenth the amount of this same MAb. These results indicate that currently available anti-TCR V region MAbs may not react consistently with T cell clones expressing the corresponding V region or may react with a low affinity making detection difficult. Differences in the J-C junction or in CDR3 may influence the binding of these MAbs. Until the false negative rate is reduced and the fine specificity and affinity of these MAbs is better characterized, both PCR and MAb studies will be required to reliably identify and quantitate clonal T cell populations.

摘要

已证明,与人T细胞受体(TCR)Vβ或Vα区域反应的单克隆抗体(MAb)在识别T细胞克隆方面几乎与个体独特型单克隆抗体一样具有特异性。如果有Vβ特异性单克隆抗体,无需聚合酶链反应(PCR)技术来评估Vβ基因家族的表达,就可以通过免疫荧光分析轻松地识别和定量扩增的恶性或非恶性T细胞群体。采用逆转录酶(RT)-PCR分析了23例连续性Sezary综合征患者外周血淋巴细胞的Vβ表达情况。10例患者有表达与市售抗Vβ抗体相对应的TCR Vβ的恶性T细胞克隆。用抗Vβ单克隆抗体进行免疫荧光染色显示,10例患者中有7例与RT-PCR结果直接相关。用任何单克隆抗体进行免疫荧光染色均未发现假阳性反应。然而,3例患者的细胞与相应的抗Vβ单克隆抗体不发生反应。这3例表达了来自含单个成员的基因家族的TCR Vβ,即Vβ14、Vβ18和Vβ20,但据报道对这些区域具有特异性的单克隆抗体未能与这些患者的T细胞克隆发生反应。对这些病例中PCR产物的测序证实了RT-PCR结果。2例患者的细胞使用具有不同J-C片段的Vβ5.1-Dβ1.1基因表达TCR。1例患者的细胞与抗Vβ5.1单克隆抗体(LC4)发生反应,而另1例患者的细胞结合的该单克隆抗体量为前者的十分之一。这些结果表明,目前可用的抗TCR V区单克隆抗体可能不会始终与表达相应V区的T细胞克隆发生反应,或者可能以低亲和力发生反应,从而使检测变得困难。J-C连接区或互补决定区3(CDR3)的差异可能会影响这些单克隆抗体的结合。在降低假阴性率并更好地表征这些单克隆抗体的精细特异性和亲和力之前,需要同时进行PCR和单克隆抗体研究,以可靠地识别和定量克隆性T细胞群体。

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