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首页> 外文期刊>Journal of cutaneous pathology >Automated kappa and lambda light chain mRNA expression for the assessment of B-cell clonality in cutaneous B-cell infiltrates: its utility and diagnostic application.
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Automated kappa and lambda light chain mRNA expression for the assessment of B-cell clonality in cutaneous B-cell infiltrates: its utility and diagnostic application.

机译:自动化的κ和λ轻链mRNA表达用于评估皮肤B细胞浸润​​中B细胞克隆性:其实用性和诊断性应用。

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摘要

INTRODUCTION: Primary cutaneous B-cell lymphoma (1 degrees CBCL) accounts for 25% of all lymphomas. The difficulty in distinction of reactive from neoplastic B-cell infiltrates prompts the use of molecular diagnostic adjuncts. While T-cell clonality can be seen in various reactive states, clonal B-cell infiltrates are often neoplastic; standard assays employed include polymerase chain reaction (PCR) or Southern blot analysis to assess heavy chain rearrangement. We sought to assess the utility of kappa (kappa) and lambda (lambda) mRNA expression using the Ventana automated assay (Ventana Medical Systems, Tucson, AZ, USA) in the analysis of atypical cutaneous B-cell lymphoid infiltrates. MATERIALS AND METHODS: Multiple 4 micro m sections of paraffin-embedded, formalin-fixed skin biopsies from 31 patients with CBCL were placed on silane-coated slides, deparaffinized, then digested in pepsin (5 mg/ml) for 30 min at 37 degrees C. Fluorescein-tagged oligoprobes and tissue mRNA were denatured at 80 degrees C for 5 min, hybridized for 2 h at 37 degrees C, and incubated with antifluorescein alkaline phosphatase conjugates. Detection of the probe target complex employed nitroblue tetrazolium and bromochloroindolyl phosphate conjugates with a nuclear fast red counterstain. A kappa : lambda ratio > 3 : 1 was held to represent kappa light chain restriction and a kappa : lambda ratio
机译:简介:原发性皮肤B细胞淋巴瘤(1度CBCL)占所有淋巴瘤的25%。区分反应性和肿瘤性B细胞浸润​​的困难,促使使用分子诊断辅助剂。虽然可以在各种反应状态下看到T细胞克隆性,但克隆性B细胞浸润​​通常是肿瘤性的。所采用的标准测定方法包括聚合酶链反应(PCR)或Southern blot分析,以评估重链重排。我们试图使用Ventana自动测定法(Ventana Medical Systems,图森,亚利桑那州,美国)评估非典型皮肤B细胞淋巴样浸润中的κ和λmRNA表达。材料与方法:将31例CBCL患者的石蜡包埋的,福尔马林固定的皮肤活检样本的4微米切片,放在涂有硅烷的载玻片上,脱蜡,然后在胃蛋白酶(5 mg / ml)中于37度消化30分钟C.将荧光素标记的寡探针和组织mRNA在80℃下变性5分钟,在37℃下杂交2小时,并与抗荧光素碱性磷酸酶缀合物一起孵育。探针目标复合物的检测使用硝基蓝四唑鎓和溴氯吲哚磷酸酯结合物,并带有核牢牢红色复染物。保持κ∶λ之比> 3∶1代表κ轻链限制,κ∶λ之比

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