前哨淋巴结:分子研究中黑色素瘤微转移的检测。

Valeria C Denninghoff, Andrea G Kahn, Jorge Falco, Hector P Curutchet, Boris Elsner
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引用次数: 30

摘要

淋巴结状态是皮肤恶性黑色素瘤患者最重要的预后因素。临床淋巴结阳性(III期)患者应行治疗性淋巴结切除术;然而,对于临床检查呈阴性(I期和II期)的局部病变患者,手术入路仍存在争议。选择性淋巴结切除术包括术中识别淋巴结池中的第一个淋巴结,前哨淋巴结(SLN)。常规检查、连续切片和免疫组织化学可能低估肿瘤细胞的存在。PCR是一种分子生物学技术,可用于恶性黑色素瘤淋巴结转移的检测。目的:本研究的目的是利用酪氨酸酶信使RNA (mRNA)扩增技术检测新鲜冷冻sln的微转移。方法:选取42例恶性黑色素瘤患者的46份苏木精-伊红(HE)阴性前哨淋巴结标本。用S-100蛋白和HMB-45对福尔马林固定石蜡包埋切片进行免疫染色。节点的中心部分提交PCR。该方法通过酪氨酸酶互补DNA的反转录扩增和双轮PCR(巢式逆转录酶[RT]-PCR)相结合来完成。结果:在42例sln阴性患者中,有1例免疫组化染色检测到微转移灶。在分子生物学方面,42例SLN患者中有14例阳性(33%);在另外12例(29%)中,只有巢式RT-PCR阳性。将42例患者中的24例分为3组,随访5年,每组分别为1例、7例和16例。第一组包括1名患者,他提供了2份SLN样本,使用免疫组织化学染色和巢式RT-PCR两种技术均发现SLN阳性(他有肝转移,在诊断后24个月死亡)。第二组,只有巢式RT-PCR阳性SLN样本,包括12名患者中的7名,中位生存期为37个月;4名患者死于广泛的转移性疾病,其他3名患者无事件生存,但1名患者因检测阳性而同意接受治疗性淋巴结切除术。最后一组包括32例患者中的16例,完成5年生存期,两种技术,免疫组织化学染色和巢式RT-PCR均为sln阴性。16例患者中有14例(88%)在随访期间无事件生存,2例局部复发。结论:酪氨酸酶mRNA扩增可能是利用分子生物学技术检测新鲜冷冻sln微转移的一个阴性预后因素。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Sentinel lymph node: detection of micrometastases of melanoma in a molecular study.

Introduction: Lymph node status in patients with cutaneous malignant melanoma is the most important prognostic factor. Patients with clinically positive nodes (stage III) should undergo therapeutic lymphadenectomy; however, the surgical approach to the regional disease in patients with negative clinical examination (stage I and II) is still controversial. Selective lymphadenectomy consists of the intraoperative identification of the first node in the nodal basin, the sentinel lymph node (SLN). Routine examination, serial sectioning, and immunohistochemistry may underestimate the presence of tumor cells. PCR is a molecular biology technique that may be useful for the detection of malignant melanoma nodal metastases in the SLN.

Aim: The aim of this study was to use tyrosinase messenger RNA (mRNA) amplification for the detection of micrometastases in fresh frozen SLNs.

Methods: 46 hematoxylin-eosin (HE)-negative sentinel node samples from 42 patients with malignant melanoma were included in this study. Formalin-fixed paraffin-embedded sections were immunostained with S-100 protein and HMB-45. A central portion of the node was submitted for PCR. This method was accomplished with a combination of reverse transcription and amplification of the tyrosinase complementary DNA and double- round PCR (nested reverse transcriptase [RT]-PCR).

Results: In 1 of the 42 SLN-negative patients, immunohistochemistry stains allowed the detection of micrometastases. With molecular biology, 14 of the 42 SLN patients were positive (33%); in another 12 (29%), only the nested RT-PCR was positive. Of the 42 patients, 24 were put into 3 groups and followed for a 5-year period with 1, 7, and 16 patients, respectively, in the groups. The first group involved 1 patient who had provided 2 SLN samples that were found to be SLN-positive using both techniques, immunohistochemistry stains and nested RT-PCR (he had hepatic metastasis and died 24 months after diagnosis). The second group, with only nested RT-PCR positive SLN samples, included 7 of 12 patients who were followed and had a median survival of 37 months; 4 died of widespread metastatic disease, the other 3 patients had event-free survival, but 1 consented to undergo a therapeutic lymphadenectomy as a result of a positive test. The last group consisting of 16 of 32 patients, with complete 5-year survival, who were SLN-negative with both techniques, immunohistochemistry stains and nested RT-PCR. Fourteen of the 16 (88%) were event-free survival during the follow-up, and 2 had local relapse.

Conclusion: Tyrosinase mRNA amplification may be a negative prognostic factor for the detection of micrometastases in fresh frozen SLNs using molecular biology techniques.

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