首页> 外文期刊>The Journal of dermatology >Analysis of T-cell antigen receptor gamma chain gene rearrangement by polymerase chain reaction in combination with denaturing gradient gel electrophoresis in the differential diagnosis of cutaneous T-lymphoproliferative diseases.
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Analysis of T-cell antigen receptor gamma chain gene rearrangement by polymerase chain reaction in combination with denaturing gradient gel electrophoresis in the differential diagnosis of cutaneous T-lymphoproliferative diseases.

机译:聚合酶链反应与变性梯度凝胶电泳相结合的T细胞抗原受体γ链基因重排分析在皮肤T淋巴细胞增生性疾病的鉴别诊断中。

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摘要

A polymerase chain reaction (PCR)-based strategy has been developed for analysis of clonal rearrangement of the T-cell receptor gamma gene (TCR gamma) and was shown to be useful for detection of clonal T-cell populations. In this study, we performed PCR combined with denaturing gradient gel electrophoresis (DGGE) on fresh frozen biopsy samples from 16 patients with cutaneous T-lymphoproliferative diseases in whom a definite diagnosis was difficult to make on morphological and immunohistochemical grounds alone. Ages of the patients at biopsy ranged from 28 to 81 (median 62) years, and the subjects consisted of 8 men and 8 women. They presented with erythema on the extremities in 5 cases, trunk in 7, buttock in 2, and papules on the trunk and face in one case each. Clonal rearrangement of TCR gamma was observed in 3 of 16 cases. Clinical diagnoses of these three cases were mycosis fungoides, cutaneous invasion of adult T-cell leukemia (ATL), and large granular lymphocytic leukemia (LGL) of T-cell type, respectively, but they were histologically difficult to differentiate from reactive cutaneous T-cell proliferation. The skin lesions of the LGL case worsened, and this patient died two years after biopsy. Another patient with suspected mycosis fungoides in the plaque stage died due to dissemination of tumors 22 months after biopsy. The remaining one patient with ATL survived with cutaneous lesions for over four years. Clonality was not demonstrated in the remaining 13 cases, and their clinical courses were favorable. These findings showed that demonstration of clonal TCR gamma gene rearrangement using the PCR-DGGE method is very helpful for diagnosis of cutaneous T-cell neoplasms.
机译:已开发出一种基于聚合酶链反应(PCR)的策略来分析T细胞受体伽马基因(TCR gamma)的克隆重排,并已证明可用于检测克隆T细胞群体。在这项研究中,我们对16例皮肤T淋巴细胞增生性疾病的新鲜冷冻活检样本进行了PCR结合变性梯度凝胶电泳(DGGE)的研究,这些患者仅凭形态学和免疫组织化学就很难做出明确的诊断。活检患者的年龄为28至81岁(中位数为62岁),受试者包括8名男性和8名女性。他们在四肢出现红斑5例,躯干7例,臀部2例,躯干和面部丘疹分别1例。 16例中的3例观察到TCRγ的克隆重排。这三例的临床诊断分别是真菌病,蕈样肉芽肿,成人T细胞白血病(ATL)皮肤浸润和T细胞型大颗粒淋巴细胞白血病(LGL),但从组织学上讲它们很难与反应性皮肤T-细胞增殖。 LGL病例的皮肤病变加重,该患者在活检后两年死亡。另一位斑块期疑似真菌病真菌病患者因活检后22个月肿瘤扩散而死亡。剩下的一名ATL患者幸存了皮肤损伤四年以上。其余13例未显示出克隆性,其临床过程良好。这些发现表明,使用PCR-DGGE方法进行的克隆性TCRγ基​​因重排的证明对皮肤T细胞肿瘤的诊断非常有帮助。

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