Molecular history of Richter syndrome: origin from a cell already present at the time of chronic lymphocytic leukemia diagnosis

被引:23
作者
Rossi, Davide [1 ]
Spina, Valeria [1 ]
Forconi, Francesco [2 ,3 ]
Capello, Daniela [1 ]
Fangazio, Marco [1 ]
Rasi, Silvia [1 ]
Martini, Maurizio [4 ]
Gattei, Valter [5 ]
Ramponi, Antonio [6 ]
Larocca, Luigi M. [4 ]
Bertoni, Francesco [7 ]
Gaidano, Gianluca [1 ]
机构
[1] Amedeo Avogadro Univ Eastern Piedmont, Div Hematol, Dept Clin & Expt Med, I-28100 Novara, Italy
[2] Univ Siena, Div Hematol, I-53100 Siena, Italy
[3] AOUS, Siena, Italy
[4] Univ Cattolica Sacro Cuore, Inst Pathol, I-00168 Rome, Italy
[5] Ctr Riferimento Oncol, I-33081 Aviano, Italy
[6] Amedeo Avogadro Univ Eastern Piedmont, Div Pathol, Dept Clin & Expt Med, I-28100 Novara, Italy
[7] Oncol Inst So Switzerland IOSI, Bellinzona, Switzerland
关键词
chronic lymphocytic leukemia; Richter syndrome; immunoglobulin gene; intraclonal diversification; clonal evolution; SOMATIC MUTATION; GENE ANALYSIS; B-CELLS; LYMPHOMA; TRANSFORMATION; DIVERSIFICATION; HYPERMUTATION; EVOLUTION; RECEPTOR;
D O I
10.1002/ijc.26322
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Richter syndrome (RS) represents the transformation of chronic lymphocytic leukemia to aggressive lymphoma. We explored intraclonal diversification (ID) of immunoglobulin genes in order to (i) follow the evolutionary history of the RS clone (ii) compare the role of ID in clonally related RS vs. clonally unrelated cases. Most (10/11, 90.9%) clonally related RS stem from the predominant clone observed at CLL diagnosis. One single RS had a transformation pattern compatible with sequential evolution from a secondary CLL subclone. Once RS transformation had occurred, all secondary CLL subclones disappeared and were substituted by the dominant RS clone with its own descendants. These observations suggest that genetic lesions associated with RS transformation are acquired by a cell belonging to the original CLL clone, rather than being progressively accumulated by later CLL subclones. Accordingly, most (9/11, 81.1%) clonally related RS harbored a genetic lesion disrupting TP53 that was already present, though at subclonal levels, in 5/11 (45.5%) samples of the paired CLL phase. A fraction of clonally related RS switched off ID (4/11, 36.4%) or reduced the levels of ID (5/11, 45.4%) at transformation. Conversely, all clonally unrelated RS harbored ID and were characterized by a significantly higher mutation frequency compared to clonally related RS (median: 1.18 X 10-3 vs. 0.13 X 10-3; p =0.002). These data indicate that (i) clonally related RS stems from a cell that is already present within the initial CLL clone and (ii) clonally unrelated and clonally related RS are biologically distinct disorders also in terms of antigen affinity maturation.
引用
收藏
页码:3006 / 3010
页数:5
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