447:循环TP53肿瘤DNA作为子宫平滑肌肉瘤术前鉴别的潜在生物标志物

J. Lopategui, Bonnie L. Balzer, Yizhou Wang, C. Santiskulvong, Carissa A. Hyunh, Chun Yat Ong, M. Araña, M. Gayhart, F. Amersi, A. Silberman
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Thus, there is a considerable need for a reliable preoperative test to triage patients into the proper surgical procedure for LMS. TP53 alterations are reportedly associated with uterine LMS in about 40% of cases. We screened plasma for TP53 variants in patients with pathologically confirmed LMS. We evaluated TP53 circulating tumor DNA (ctDNA) by deep next-generation sequencing in a cohort of 7 patients with LMS, 1 patient with STUMP, and 3 patients with LM. Clinical data were reviewed to assess disease burden. LMS patients9 tumor burden ranged from no evidence to extensive metastatic disease. DNA extraction was performed using the QIAamp DNA Micro Kit, QIAamp DNA FFPE Tissue Kit, or QIAamp MinElute ccfDNA Mini Kit. DNA quality was assessed using the TapeStation Genomic DNA kit. NGS libraries targeting the entire exonic region of the p53 gene were prepared using the QIASeq Targeted DNA Custom Panel. Sequencing was performed on the MiSeq system using 150bp paired end sequencing with a minimum read depth of 2x0.5M reads for plasma and 2x1M reads for formalin-fixed paraffin embedded and fresh-frozen tissue samples. Raw sequencing data were demultiplexed by bcl2fastq to generate the FASTQ files. Then raw sequencing reads were aligned to the human reference genome GRCh38 by BWA-MEM 0.7.9a-r786. SmCounter2 was used for p53 variants calling and variants quality control. We discovered TP53 ctDNA variants in 5 of 7 (71.4%) LMS cases including p.E258V, p.R248Q, P.R337C, p.E221*, p.R174_R175delinsWC, but not in the control cases of LM or STUMP. In the 5 plasma samples with TP53 mutated LMS, the patients had extensive metastatic disease and in the 2 TP53 wild-type LMS and STUMP cases, the patients had no evidence of disease. To our knowledge, this is the first pilot study to demonstrate the comparative use of TP53 ctDNA in patients with LMS, LM, and STUMP. Further study of these rare LMS is needed to determine the preoperative utility of NGS TP53 ctDNA mutational status as a useful molecular biomarker to help guide surgery and avoid unwarranted manipulation and pelvic contamination of undetected LMS. Supported by the Gottlieb, Buss and Snyder Endowments in Surgical Oncology Citation Format: Jean R. Lopategui, Bonnie Balzer, Yizhou Wang, Chintda Santiskulvong, Carissa A. Hyunh, Chun Yat Ong, Manuel Arana, Matthew Gayhart, Farin Amersi, Allan W. Silberman. Circulating TP53 tumor DNA as a potential biomarker for pre-operative identification of uterine leiomyosarcoma [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. 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引用次数: 0

摘要

子宫平滑肌肉瘤(LMS)是一种高度侵袭性但罕见的恶性肿瘤,预后不佳。在几乎所有的病例中,在切除平滑肌瘤之前,LMS是不被怀疑的。据报道,在一项最大的队列研究中,隐性子宫LMS的风险为0.2%(1 / 500)。主要的问题是,术前没有可靠的方法来区分LMS与平滑肌瘤(LM)或STUMP(恶性潜能不确定的平滑肌肿瘤),如果在LM手术中发生肿瘤横切,LMS患者的预后更差。LMS缺乏有效的治疗方法,大多数患者最终死于这种疾病。因此,有相当大的需要一个可靠的术前检查,以分类患者进入适当的手术程序LMS。据报道,约40%的子宫LMS病例与TP53改变有关。我们在病理证实的LMS患者中筛查血浆TP53变异。我们对7例LMS患者、1例STUMP患者和3例LM患者的TP53循环肿瘤DNA (ctDNA)进行了深度下一代测序。回顾临床资料以评估疾病负担。LMS患者的肿瘤负荷范围从无证据到广泛的转移性疾病。采用QIAamp DNA Micro Kit、QIAamp DNA FFPE Tissue Kit或QIAamp MinElute ccfDNA Mini Kit进行DNA提取。使用TapeStation基因组DNA试剂盒评估DNA质量。使用QIASeq Targeted DNA Custom Panel制备针对p53基因整个外显子区域的NGS文库。在MiSeq系统上进行测序,采用150bp配对末端测序,血浆样品最小读取深度为2x0.5M,福尔马林固定石蜡包埋和新鲜冷冻组织样品最小读取深度为2x1M。原始测序数据通过bcl2fastq解复用生成FASTQ文件。然后用BWA-MEM 0.7.9a-r786将原始测序reads与人类参考基因组GRCh38进行比对。SmCounter2用于p53变异体的调用和变异体的质量控制。我们在7例LMS病例中发现了5例(71.4%)TP53 ctDNA变异,包括p.E258V、p.R248Q、P.R337C、p.E221*、p.R174_R175delinsWC,但在LM或STUMP的对照病例中没有发现TP53 ctDNA变异。在5例TP53突变LMS的血浆样本中,患者有广泛的转移性疾病,在2例TP53野生型LMS和STUMP病例中,患者无疾病证据。据我们所知,这是第一个证明TP53 ctDNA在LMS、LM和STUMP患者中比较使用的初步研究。需要对这些罕见的LMS进行进一步的研究,以确定NGS TP53 ctDNA突变状态作为一种有用的分子生物标志物,帮助指导手术,避免对未检测到的LMS进行不必要的操作和盆腔污染。引用格式:Jean R. Lopategui, Bonnie Balzer, yzhou Wang, Chintda Santiskulvong, Carissa A. Hyunh, Chun Yat Ong, Manuel Arana, Matthew Gayhart, Farin Amersi, Allan W. Silberman。循环TP53肿瘤DNA作为子宫平滑肌肉瘤术前鉴别的潜在生物标志物[摘要]。见:美国癌症研究协会2021年年会论文集;2021年4月10日至15日和5月17日至21日。费城(PA): AACR;癌症杂志,2021;81(13 -增刊):447。
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Abstract 447: Circulating TP53 tumor DNA as a potential biomarker for pre-operative identification of uterine leiomyosarcoma
Uterine leiomyosarcoma (LMS) is a highly aggressive but rare malignancy with a dismal prognosis. In nearly all cases, LMS is unsuspected prior to resection for a presumed leiomyoma. The risk of occult uterine LMS is reported to be 0.2% (1 in 500) in the largest cohort study of women undergoing surgery for presumed fibroid disease. The major problem is that there is no reliable preoperative method to distinguish LMS from a leiomyoma (LM) or STUMP (smooth muscle tumor of uncertain malignant potential), and the patient9s prognosis for LMS is even poorer if the tumor is transected, which occurs in procedures performed for LM. Effective therapy for LMS is lacking and most patients eventually succumb to the disease. Thus, there is a considerable need for a reliable preoperative test to triage patients into the proper surgical procedure for LMS. TP53 alterations are reportedly associated with uterine LMS in about 40% of cases. We screened plasma for TP53 variants in patients with pathologically confirmed LMS. We evaluated TP53 circulating tumor DNA (ctDNA) by deep next-generation sequencing in a cohort of 7 patients with LMS, 1 patient with STUMP, and 3 patients with LM. Clinical data were reviewed to assess disease burden. LMS patients9 tumor burden ranged from no evidence to extensive metastatic disease. DNA extraction was performed using the QIAamp DNA Micro Kit, QIAamp DNA FFPE Tissue Kit, or QIAamp MinElute ccfDNA Mini Kit. DNA quality was assessed using the TapeStation Genomic DNA kit. NGS libraries targeting the entire exonic region of the p53 gene were prepared using the QIASeq Targeted DNA Custom Panel. Sequencing was performed on the MiSeq system using 150bp paired end sequencing with a minimum read depth of 2x0.5M reads for plasma and 2x1M reads for formalin-fixed paraffin embedded and fresh-frozen tissue samples. Raw sequencing data were demultiplexed by bcl2fastq to generate the FASTQ files. Then raw sequencing reads were aligned to the human reference genome GRCh38 by BWA-MEM 0.7.9a-r786. SmCounter2 was used for p53 variants calling and variants quality control. We discovered TP53 ctDNA variants in 5 of 7 (71.4%) LMS cases including p.E258V, p.R248Q, P.R337C, p.E221*, p.R174_R175delinsWC, but not in the control cases of LM or STUMP. In the 5 plasma samples with TP53 mutated LMS, the patients had extensive metastatic disease and in the 2 TP53 wild-type LMS and STUMP cases, the patients had no evidence of disease. To our knowledge, this is the first pilot study to demonstrate the comparative use of TP53 ctDNA in patients with LMS, LM, and STUMP. Further study of these rare LMS is needed to determine the preoperative utility of NGS TP53 ctDNA mutational status as a useful molecular biomarker to help guide surgery and avoid unwarranted manipulation and pelvic contamination of undetected LMS. Supported by the Gottlieb, Buss and Snyder Endowments in Surgical Oncology Citation Format: Jean R. Lopategui, Bonnie Balzer, Yizhou Wang, Chintda Santiskulvong, Carissa A. Hyunh, Chun Yat Ong, Manuel Arana, Matthew Gayhart, Farin Amersi, Allan W. Silberman. Circulating TP53 tumor DNA as a potential biomarker for pre-operative identification of uterine leiomyosarcoma [abstract]. In: Proceedings of the American Association for Cancer Research Annual Meeting 2021; 2021 Apr 10-15 and May 17-21. Philadelphia (PA): AACR; Cancer Res 2021;81(13_Suppl):Abstract nr 447.
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