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结节性淋巴细胞为主型霍奇金淋巴瘤合并大细胞淋巴瘤:通过V-J聚合酶链反应分析Ig基因重排

Nodular lymphocyte-predominant Hodgkin's disease associated with large-cell lymphoma: analysis of Ig gene rearrangements by V-J polymerase chain reaction.

作者信息

Greiner T C, Gascoyne R D, Anderson M E, Kingma D W, Adomat S A, Said J, Jaffe E S

机构信息

Laboratory of Pathology, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892-1500, USA.

出版信息

Blood. 1996 Jul 15;88(2):657-66.

PMID:8695813
Abstract

The clonality of nodular lymphocyte-predominant Hodgkin's disease (NLPHD) and the relationship to composite or sequential large-cell lymphomas (LCLs) is poorly understood. Clonal Ig heavy-chain gene rearrangements (lgHGR) have infrequently been observed in NLPHD by Southern hybridization. The goals of this study were (1) to determine if IgHGR could be identified by polymerase chain reaction (PCR) techniques in the LCL associated with NLPHD; (2) to determine if the lgHGR identified in the LCL could also be found in the associated NLPHD; and (3) to determine if Epstein-Barr virus (EBV) played a role a role in histologic progression to LCL. Using consensus primers to conserved regions in the lgH variable (V) and joining (J) region genes, we analyzed formalin-fixed paraffin-embedded sections from the biopsies of 25 patients referred to the National Cancer Institute (NCI) registry for NLPHD and LCL using both single-step and seminested V-J PCR. The histologically aggressive component was further subclassified as frank LCL or as L&H-cell-rich, but not fulfilling criteria for LCL. Matched samples representing both NLPHD and aggressive components were available in 13 cases. In 12 cases, only one component was available (aggressive, n = 8; NLPHD, n = 4). In addition, we also amplified, with 32P labeling, 12 cases of NLPHD without associated LCL. Two clonal IgHGR were identified in 29 cases (7%) of typical NLPHD, both of which were associated with LCL containing a similar sized band by PCR. The clonal identity of the bands in the NLPHD and associated LCL was confirmed by sequencing the products in these two cases. Eight of 10 cases (80%) of LCL associated with NLPHD contained a clonal band by this technique. By contrast, none of the cases classified as L&H-cell-rich contained an IgHGR. The single-step and seminested PCR methods produced identical results. All clonal LCLs were studied for EBV sequences by in situ hybridization using the EBER1 probe, and were negative. We conclude that the LCLs associated with NLPHD are clonal B-cell malignancies. However, by these methods, the same clone can be identified in only a minority of cases of NLPHD and LCL. EBV does not appear to play a role in histologic progression. Moreover, our results suggest that many cases suspected of being LCL may actually represent NLPHD with increased numbers of L&H cells. In histologically equivocal cases, the diagnosis of LCL should be reserved for those cases in which a clonal B-cell neoplasm can be demonstrated.

摘要

结节性淋巴细胞为主型霍奇金淋巴瘤(NLPHD)的克隆性及其与复合性或序贯性大细胞淋巴瘤(LCL)的关系尚不清楚。通过Southern杂交在NLPHD中很少观察到克隆性免疫球蛋白重链基因重排(IgHGR)。本研究的目的是:(1)确定是否可以通过聚合酶链反应(PCR)技术在与NLPHD相关的LCL中鉴定出IgHGR;(2)确定在LCL中鉴定出的IgHGR是否也能在相关的NLPHD中找到;(3)确定爱泼斯坦-巴尔病毒(EBV)在向LCL的组织学进展中是否起作用。使用针对免疫球蛋白可变(V)区和连接(J)区基因保守区域的共有引物,我们采用单步和半巢式V-J PCR分析了来自转诊至美国国立癌症研究所(NCI)登记处的25例NLPHD和LCL患者活检组织的福尔马林固定石蜡包埋切片。组织学上侵袭性成分进一步细分为明确的LCL或富含L&H细胞但不符合LCL标准的类型。13例患者有代表NLPHD和侵袭性成分的配对样本。12例患者仅有一种成分(侵袭性成分,n = 8;NLPHD,n = 4)。此外,我们还用32P标记扩增了12例无相关LCL的NLPHD。在29例(7%)典型NLPHD中鉴定出两个克隆性IgHGR,通过PCR发现这两个克隆性IgHGR均与含有相似大小条带的LCL相关。通过对这两例产物进行测序,证实了NLPHD和相关LCL中条带的克隆一致性。通过该技术,10例与NLPHD相关的LCL中有8例(80%)含有克隆条带。相比之下,所有分类为富含L&H细胞的病例均未检测到IgHGR。单步和半巢式PCR方法产生相同的结果。所有克隆性LCL均使用EBER1探针通过原位杂交研究EBV序列,结果均为阴性。我们得出结论,与NLPHD相关的LCL是克隆性B细胞恶性肿瘤。然而,通过这些方法,仅在少数NLPHD和LCL病例中能鉴定出相同的克隆。EBV似乎在组织学进展中不起作用。此外,我们的结果表明,许多疑似LCL的病例实际上可能是L&H细胞数量增加的NLPHD。在组织学不明确的病例中,LCL的诊断应仅限于那些能证明存在克隆性B细胞肿瘤的病例。

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