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A der(8)t(8;11) chromosome in the Karpas-620 myeloma cell line expresses only Cyclin D1: Yet both Cyclin D1 and MYC are repositioned in close proximity to the 3′ IGH enhancer

机译:Karpas-620骨髓瘤细胞系中的der(8)t(8; 11)染色体仅表达细胞周期蛋白D1:而细胞周期蛋白D1和MYC都重新定位在3IGH增强子附近

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摘要

The Karpas-620 human myeloma cell line (HMCL) expresses high levels of Cyclin D1 (CCND1), but has a der(8)t(8;11) and a der(14)t(8;14), and not a conventional t(11;14). Fluorescent in situ hybridization (FISH) and array comparative genomic hybridization (aCGH) studies suggest that der(14)t(11;14) from a primary translocation underwent a secondary translocation with chromosome 8 to generate der(8)t(8;[14];11) and der(14)t(8;[11];14). Both secondary derivatives share extensive identical sequences from chromosomes 8, 11, and 14, including MYC and the 3′ IgH enhancers. Der(14), with MYC located ~700 kb telomeric to the 3′ IGH enhancer, expresses MYC. By contrast, der(8), with both CCND1 and MYC repositioned near a 3′ IGH enhancer, expresses CCND1, which is telomeric of the enhancer, but not MYC, which is centromeric to the enhancer. The secondary translocation that dysregulated MYC resulted in extensive regions from both donor chromosomes being transmitted to both derivative chromosomes, suggesting a defect in DNA recombination or repair in the myeloma tumor cell.
机译:Karpas-620人骨髓瘤细胞系(HMCL)表达高水平的Cyclin D1(CCND1),但具有der(8)t(8; 11)和der(14)t(8; 14),而并非传统的t(11; 14)。荧光原位杂交(FISH)和阵列比较基因组杂交(aCGH)研究表明,一次易位的der(14)t(11; 14)经历了8号染色体的二次易位,产生了der(8)t(8; [ 14]; 11)和der(14)t(8; [11]; 14)。两种次级衍生物都具有来自染色体8、11和14的广泛相同序列,包括MYC和3'IgH增强子。 MYC位于3'IGH增强子的约700 kb端粒的Der(14)表达MYC。相反,将CCND1和MYC都重新定位在3'IGH增强子附近的der(8)表达CCND1,它是增强子的端粒,而不是MYC,它是增强子的着丝粒。 MYC失调的继发易位导致两个供体染色体的广泛区域被传递到两个衍生染色体,表明骨髓瘤肿瘤细胞的DNA重组或修复缺陷。

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