关键词: RT-qPCR alveolar rhabdomyosarcoma formalin-fixed paraffin-embedded (FFPE) tissue fusion gene fusion transcript mRNA capture sequencing sarcoma undifferentiated round cell sarcoma

Mesh : Adaptor Protein Complex 1 / genetics Adaptor Protein Complex beta Subunits Cell Cycle Proteins / genetics Dithionitrobenzoic Acid Humans In Situ Hybridization, Fluorescence Nuclear Proteins / genetics Oncogene Proteins, Fusion / genetics RNA RNA, Messenger / genetics Reverse Transcriptase Polymerase Chain Reaction Sarcoma / diagnosis genetics pathology Soft Tissue Neoplasms / pathology Transcription Factors / genetics

来  源:   DOI:10.3390/ijms231911007

Abstract:
We assess the performance of mRNA capture sequencing to identify fusion transcripts in FFPE tissue of different sarcoma types, followed by RT-qPCR confirmation. To validate our workflow, six positive control tumors with a specific chromosomal rearrangement were analyzed using the TruSight RNA Pan-Cancer Panel. Fusion transcript calling by FusionCatcher confirmed these aberrations and enabled the identification of both fusion gene partners and breakpoints. Next, whole-transcriptome TruSeq RNA Exome sequencing was applied to 17 fusion gene-negative alveolar rhabdomyosarcoma (ARMS) or undifferentiated round cell sarcoma (URCS) tumors, for whom fluorescence in situ hybridization (FISH) did not identify the classical pathognomonic rearrangements. For six patients, a pathognomonic fusion transcript was readily detected, i.e., PAX3-FOXO1 in two ARMS patients, and EWSR1-FLI1, EWSR1-ERG, or EWSR1-NFATC2 in four URCS patients. For the 11 remaining patients, 11 newly identified fusion transcripts were confirmed by RT-qPCR, including COPS3-TOM1L2, NCOA1-DTNB, WWTR1-LINC01986, PLAA-MOB3B, AP1B1-CHEK2, and BRD4-LEUTX fusion transcripts in ARMS patients. Additionally, recurrently detected secondary fusion transcripts in patients diagnosed with EWSR1-NFATC2-positive sarcoma were confirmed (COPS4-TBC1D9, PICALM-SYTL2, SMG6-VPS53, and UBE2F-ALS2). In conclusion, this study shows that mRNA capture sequencing enhances the detection rate of pathognomonic fusions and enables the identification of novel and secondary fusion transcripts in sarcomas.
摘要:
我们评估了mRNA捕获测序的性能,以鉴定不同肉瘤类型的FFPE组织中的融合转录本,然后进行RT-qPCR确认。要验证我们的工作流程,使用TruSightRNA泛癌症小组分析了6种具有特定染色体重排的阳性对照肿瘤.FusionCatcher的融合转录物调用证实了这些畸变,并能够鉴定融合基因伴侣和断点。接下来,全转录组TruSeqRNA外显子组测序应用于17个融合基因阴性的肺泡横纹肌肉瘤(ARMS)或未分化的圆形细胞肉瘤(URCS)肿瘤,荧光原位杂交(FISH)未能鉴定出经典的病理学重排.对于六个病人来说,很容易检测到病态融合转录本,即,两名ARMS患者的PAX3-FOXO1,和EWSR1-FLI1,EWSR1-ERG,或EWSR1-NFATC2在四名URCS患者中。对于剩下的11名患者,通过RT-qPCR确认了11个新鉴定的融合转录本,包括COPS3-TOM1L2,NCOA1-DTNB,WWTR1-LINC01986,PLAA-MOB3B,ARMS患者的AP1B1-CHEK2和BRD4-LEUTX融合转录本。此外,在诊断为EWSR1-NFATC2阳性肉瘤的患者中反复检测到的次级融合转录本得到证实(COPS4-TBC1D9,PICALM-SYTL2,SMG6-VPS53和UBE2F-ALS2).总之,这项研究表明,mRNA捕获测序提高了病理基因融合的检出率,并能够鉴定肉瘤中的新的和次级融合转录本。
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