Department of Pathology, Amsterdam University Medical Center, Location AMC, University of Amsterdam, Lymphoma and Myeloma Center Amsterdam (LYMMCARE), Amsterdam, The Netherlands.
Laboratory of Experimental Cardiology, University Medical Center Utrecht, Utrecht University, Utrecht, The Netherlands.
Eur J Immunol. 2024 Oct;54(10):e2350958. doi: 10.1002/eji.202350958. Epub 2024 Jul 24.
In developing B cells, V(D)J gene recombination is initiated by the RAG1/2 endonuclease complex, introducing double-stranded DNA breaks (DSBs) in V, D, and J genes and resulting in the formation of the hypervariable parts of immunoglobulins (Ig). Persistent or aberrant RAG1/2 targeting is a potential threat to genome integrity. While RAG1 and RAG2 have been shown to bind various regions genome-wide, the in vivo off-target DNA damage instigated by RAG1/2 endonuclease remains less well understood. In the current study, we identified regions containing RAG1/2-induced DNA breaks in mouse pre-B cells on a genome-wide scale using a global DNA DSB detection strategy. We detected 1489 putative RAG1/2-dependent DSBs, most of which were located outside the Ig loci. DNA sequence motif analysis showed a specific enrichment of RAG1/2-induced DNA DSBs at GA- and CA-repeats and GC-rich motifs. These findings provide further insights into RAG1/2 off-target activity. The ability of RAG1/2 to introduce DSBs on the non-Ig loci during the endogenous V(D)J recombination emphasizes its genotoxic potential in developing lymphocytes.
在 B 细胞发育过程中,RAG1/2 内切酶复合物启动 V(D)J 基因重排,在 V、D 和 J 基因中引入双链 DNA 断裂(DSB),从而形成免疫球蛋白(Ig)的超变区。持续或异常的 RAG1/2 靶向是对基因组完整性的潜在威胁。虽然 RAG1 和 RAG2 已被证明可以结合全基因组的各种区域,但 RAG1/2 内切酶引发的体内非靶标 DNA 损伤仍了解较少。在本研究中,我们使用全基因组 DSB 检测策略,在小鼠前 B 细胞中鉴定出 RAG1/2 诱导的全基因组范围内的 DNA 断裂区域。我们检测到 1489 个疑似 RAG1/2 依赖性 DSB,其中大多数位于 Ig 基因座之外。DNA 序列基序分析显示,GA 和 CA 重复序列和富含 GC 的基序特异性富集了 RAG1/2 诱导的 DNA DSB。这些发现为 RAG1/2 非靶标活性提供了进一步的见解。RAG1/2 在内源 V(D)J 重排过程中在非 Ig 基因座上引入 DSB,强调了其在发育淋巴细胞中的遗传毒性潜力。
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