Combination of Complement-Dependent Cytotoxicity and Relative Fluorescent Quantification of HLA Length Polymorphisms Facilitates the Detection of a Loss of Heterozygosity.

Bone Marrow Research Pub Date : 2014-01-01 Epub Date: 2014-04-03 DOI:10.1155/2014/541345
Klaus Witter, Roland Reibke, Marion Subklewe, Robert Zahn, Teresa Kauke, Karsten Spiekermann, Michael Spannagl, Johanna Tischer, Wolfgang Hiddemann, Andrea Dick
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Abstract

Loss of heterozygosity (LOH) is a common event in malignant cells. In this work we introduce a new approach to identify patients with loss of heterozygosity in the HLA region either at first diagnosis or after HLA mismatched allogeneic HSCT. Diagnosis of LOH requires a high purity of recipient target cells. FACS is time consuming and also frequently prevented by rather nonspecific or unknown immune phenotype. The approach for recipient cell enrichment is based on HLA targeted complement-dependent cytotoxicity (CDC). Relative fluorescent quantification (RFQ) analysis of HLA intron length polymorphisms then allows analysis of HLA heterozygosity. The approach is exemplified in recent clinical cases illustrating the detection of an acquired allele loss. As illustrated in one case with DPB1, distinct HLA loci in donor and patient were sufficient for both proof of donor cell removal and evaluation of allele loss in the patient's leukemic cells. Results were confirmed using HLA-B RFQ analysis and leukemia-associated aberrant immunophenotype (LAIP) based cell sort. Both results confirmed suspected loss of HLA heterozygosity. Our approach complements or substitutes for FACS-based cell enrichment; hence it may be further developed as novel routine diagnostic tool. This allows rapid recipient cell purification and testing for loss of HLA heterozygosity before and after allogeneic HSCT in easily accessible peripheral blood samples.

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补体依赖性细胞毒性和HLA长度多态性的相对荧光定量相结合有助于检测杂合性缺失。
杂合性缺失(LOH)是恶性细胞中常见的事件。在这项工作中,我们介绍了一种新的方法来识别HLA区域杂合性缺失的患者,无论是在首次诊断还是在HLA不匹配的异体造血干细胞移植后。LOH的诊断需要高纯度的受体靶细胞。FACS是耗时的,也经常被非特异性或未知的免疫表型所预防。受体细胞富集的方法是基于HLA靶向补体依赖性细胞毒性(CDC)。相对荧光定量(RFQ)分析HLA内含子长度多态性,然后分析HLA杂合性。该方法在最近的临床病例中得到了例证,说明了获得性等位基因丢失的检测。如一例DPB1病例所示,供体和患者中不同的HLA位点足以证明供体细胞移除和评估患者白血病细胞中等位基因丢失。结果通过HLA-B RFQ分析和基于白血病相关异常免疫表型(LAIP)的细胞分选得到证实。这两个结果都证实了怀疑的HLA杂合性缺失。我们的方法补充或替代基于facs的细胞富集;因此,它可以进一步发展为一种新的常规诊断工具。这使得在容易获得的外周血样本中进行同种异体造血干细胞移植前后的受体细胞快速纯化和HLA杂合性缺失检测成为可能。
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