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Somatic hypermutation analysis in follicular lymphoma provides evidence suggesting bidirectional cell migration between lymph node and bone marrow during disease progression and relapse

机译:滤泡性淋巴瘤的体细胞高突变分析提供了证据表明在疾病进展和复发过程中淋巴结与骨髓之间存在双向细胞迁移

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摘要

In follicular lymphoma, somatic hypermutation of the immunoglobulin heavy chain genes facilitates the identification of different lymphoma cell clones, and the construction of genealogical trees. To investigate the dissemination of lymphoma cells, and the role of bone marrow in disease progression, we simultaneously analyzed the somatic hypermutation patterns of lymph node and bone marrow specimens taken from three patients at onset and relapse of their disease. Immunoglobulin heavy chain genes were amplified by polymerase chain reaction, cloned and sequenced. Mutational pedigrees were constructed in a hierarchical order. When direct transition of one mutation pattern into that of a successor clones was not feasible, hypothetical predecessor clones were created, and a probability measurement calculation was introduced. Eighty-five sequenced clones were generated. The average mutation rates were 13.45% for the lymph node specimens, and 9.78% for the bone marrow ones. Forty-two hypothetical predecessor clones were introduced into inter-compartment pedigrees. The genealogical trees showed that early lymphoma clones with a low mutational load quickly migrate from lymph nodes into the bone marrow. Bi-directional lymphoma cell migration was detectable between the two compartments. In one case of follicular lymphoma, a clone identical to the initial lymph node clone was detected 2 years later in the bone marrow. The newly introduced algorithm allows the evaluation of both time and direction of follicular lymphoma cell migration. We found evidence that follicular lymphoma originates in the lymph node, and infiltrates the bone marrow early in the course of the disease. Moreover, inter-compartment migration between lymph nodes and bone marrow occurs in both directions.
机译:在滤泡性淋巴瘤中,免疫球蛋白重链基因的体细胞超突变促进了不同淋巴瘤细胞克隆的鉴定和谱系树的构建。为了研究淋巴瘤细胞的分布以及骨髓在疾病进展中的作用,我们同时分析了三例患者发病和复发时淋巴结和骨髓标本的体细胞高变模式。通过聚合酶链反应扩增免疫球蛋白重链基因,进行克隆和测序。变异谱系是按层次结构构建的。当无法将一个突变模式直接转换为后继克隆的突变时,将创建假设的前代克隆,并引入概率测量计算。产生了八十五个测序克隆。淋巴结标本的平均突变率为13.45%,骨髓标本的平均突变率为9.78%。 42个假想的前代克隆被引入到室间谱系中。族谱树表明,具有低突变负荷的早期淋巴瘤克隆会迅速从淋巴结迁移到骨髓。在两个区室之间可检测到双向淋巴瘤细胞迁移。在一个滤泡性淋巴瘤病例中,两年后在骨髓中发现了与最初的淋巴结克隆相同的克隆。新引入的算法可以评估滤泡性淋巴瘤细胞迁移的时间和方向。我们发现证据表明,滤泡性淋巴瘤起源于淋巴结,并在疾病过程的早期渗入骨髓。而且,淋巴结和骨髓之间的室间迁移在两个方向上都发生。

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