Characteristics and Clinical Value of MYC, BCL2, and BCL6 Rearrangement Detected by Next-generation Sequencing in DLBCL.

Yupeng Zeng, Ran Wei, Longlong Bao, Tian Xue, Yulan Qin, Min Ren, Qianming Bai, Qianlan Yao, Chengli Yu, Chen Chen, Ping Wei, Baohua Yu, Junning Cao, Xiaoqiu Li, Qunling Zhang, Xiaoyan Zhou
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Abstract

MYC, BCL2, and BCL6 rearrangements are clinically important events of diffuse large B-cell lymphoma (DLBCL). The ability and clinical value of targeted next-generation sequencing (NGS) in the detection of these rearrangements in DLBCL have not been fully determined. We performed targeted NGS (481-gene-panel) and break-apart FISH of MYC, BCL2, and BCL6 gene regions in 233 DLBCL cases. We identified 88 rearrangements (16 MYC; 20 BCL2; 52 BCL6 ) using NGS and 96 rearrangements (28 MYC; 20 BCL2; 65 BCL6) using FISH. The consistency rates between FISH and targeted NGS for the detection of MYC, BCL2, and BCL6 rearrangements were 93%, 97%, and 89%, respectively. FISH-cryptic rearrangements (NGS+/FISH-) were detected in 7 cases (1 MYC; 3 BCL2; 2 BCL6; 1 MYC::BCL6), mainly caused by small chromosomal insertions and inversions. NGS-/FISH+ were detected in 38 cases (14 MYC; 4 BCL2; 20 BCL6).To clarify the cause of the inconsistencies, we selected 17 from the NGS-/FISH+ rearrangements for further whole genome sequencing (WGS), and all 17 rearrangements were detected with break points by WGS. These break points were all located outside the region covered by the probe of targeted NGS, and most (16/17) were located in the intergenic region. These results indicated that targeted NGS is a powerful clinical diagnostics tool for comprehensive MYC, BCL2, and BCL6 rearrangement detection. Compared to FISH, it has advantages in describing the break point distribution, identifying uncharacterized partners, and detecting FISH-cryptic rearrangements. However, the lack of high-sensitivity caused by insufficient probe coverage is the main limitation of the current technology.
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下一代测序检测到的DLBCL中MYC、BCL2和BCL6重排的特征和临床价值
MYC、BCL2 和 BCL6 重排是弥漫大 B 细胞淋巴瘤(DLBCL)的重要临床症状。靶向新一代测序(NGS)在 DLBCL 中检测这些重排的能力和临床价值尚未完全确定。我们对 233 例 DLBCL 病例的 MYC、BCL2 和 BCL6 基因区进行了靶向 NGS(481 基因面板)和断裂 FISH 检测。我们使用 NGS 发现了 88 个重排(16 个 MYC;20 个 BCL2;52 个 BCL6),使用 FISH 发现了 96 个重排(28 个 MYC;20 个 BCL2;65 个 BCL6)。FISH 和靶向 NGS 检测 MYC、BCL2 和 BCL6 重排的一致率分别为 93%、97% 和 89%。在 7 个病例(1 个 MYC;3 个 BCL2;2 个 BCL6;1 个 MYC::BCL6)中检测到 FISH 加密重排(NGS+/FISH-),主要由染色体小插入和倒位引起。为了弄清不一致的原因,我们从 NGS-/FISH+ 重排中选择了 17 个进行进一步的全基因组测序(WGS),结果发现所有 17 个重排都有 WGS 检测到的断裂点。这些断裂点全部位于靶向 NGS 探针覆盖的区域之外,其中大部分(16/17)位于基因间区。这些结果表明,靶向 NGS 是全面检测 MYC、BCL2 和 BCL6 重排的强大临床诊断工具。与 FISH 相比,它在描述断裂点分布、识别未定性伙伴和检测 FISH 加密重排方面具有优势。然而,探针覆盖率不足导致灵敏度不高是目前该技术的主要局限。
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