Kjeldsen Eigil
HemoDiagnostic Laboratory, CancerCytogenetic Section, Department of Hematology, Aarhus University Hospital, Tage-Hansens Gade 2, Ent. 4A, DK-8000 Aarhus C, Denmark.
Exp Mol Pathol. 2015 Aug;99(1):50-5. doi: 10.1016/j.yexmp.2015.05.005. Epub 2015 May 8.
Hypereosinophilic syndrome (HES) is a clinically and pathologically heterogeneous disease entity. It is characterized by persistent eosinophilia and organ damage after excluding other causes. Clonal eosinophilia is distinguished from idiopathic eosinophilia by the presence of histologic, cytogenetic, or molecular evidence of an underlying malignancy. There are two distinct subcategories of clonal eosinophilia: chronic eosinophilic leukemia, not otherwise specified and myeloid/lymphoid neoplasms with eosinophilia and mutations involving platelet-derived growth factor receptor α/β or fibroblast growth factor receptor 1. More than 50% of HES are without knowledge of underlying pathogenic molecular pathways. Here we examined a HES patient by oligo-based aCGH analysis and molecular cytogenetic methods. Examination for the common eosinophilia-related cytogenetic abnormalities involving the genes PDGFRA, PDGFRB, and FGFR1 together with BCR-ABL fusion gene was negative. Cytogenetic analysis and multi-color FISH analysis revealed a novel cryptic three-way translocation t(2;11;5)(p21.3;q13.5;q23.2). By oaCGH analysis we could not find any copy number changes related to the cytogenetic breakpoints but instead detected a 0.9Mb submicroscopic deletion at 11p14.3. The deleted region involved the 5'-upstream sequences and exons 1-4 of the LUZP2 gene, which encodes a leucine zipper protein. Analysis of surrogate germ-line cells revealed a normal result showing that the detected chromosomal aberrations were acquired. This is the first report on a HES patient associated with a novel complex three-way translocation t(2;11;5)(p21.3;q13.5;q23.2) and a submicroscopic deletion in chromosome band 11p14.3. The study also demonstrates the benefits of oligo-based aCGH analysis in detecting hidden disease related chromosomal abnormalities. The present findings provide additional clues to unravel important molecular pathways in HES to obtain the full spectrum of acquired chromosomal and genomic aberrations in this heterogeneous disease entity. As more cases become characterized this may eventually improve on classification and treatment options.
高嗜酸性粒细胞综合征(HES)是一种临床和病理上异质性的疾病实体。其特征是在排除其他病因后出现持续性嗜酸性粒细胞增多和器官损害。克隆性嗜酸性粒细胞增多症与特发性嗜酸性粒细胞增多症的区别在于存在潜在恶性肿瘤的组织学、细胞遗传学或分子证据。克隆性嗜酸性粒细胞增多症有两个不同的亚类:未另行指定的慢性嗜酸性粒细胞白血病,以及伴有嗜酸性粒细胞增多和涉及血小板衍生生长因子受体α/β或成纤维细胞生长因子受体1突变的髓系/淋巴系肿瘤。超过50%的HES患者不清楚潜在的致病分子途径。在此,我们通过基于寡核苷酸的aCGH分析和分子细胞遗传学方法对一名HES患者进行了检查。对涉及PDGFRA、PDGFRB和FGFR1基因以及BCR-ABL融合基因的常见嗜酸性粒细胞增多相关细胞遗传学异常的检测结果为阴性。细胞遗传学分析和多色FISH分析发现了一种新的隐匿性三向易位t(2;11;5)(p21.3;q13.5;q23.2)。通过oaCGH分析,我们未发现与细胞遗传学断点相关的任何拷贝数变化,但在11p14.3处检测到一个0.9Mb的亚微观缺失。缺失区域涉及LUZP2基因的5'-上游序列和外显子1-4,该基因编码一种亮氨酸拉链蛋白。对替代生殖系细胞的分析显示结果正常,表明检测到的染色体畸变是后天获得的。这是关于一名与新型复杂三向易位t(2;11;5)(p21.3;q13.5;q23.2)和11p14.3染色体带亚微观缺失相关的HES患者的首次报告。该研究还证明了基于寡核苷酸的aCGH分析在检测隐匿性疾病相关染色体异常方面的益处。目前的发现为揭示HES中重要的分子途径提供了额外线索,以获得这种异质性疾病实体中后天获得的染色体和基因组畸变的全貌。随着更多病例得到特征化,这最终可能会改善分类和治疗选择。
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