Centre for Reproductive Health, Hudson Institute of Medical Research, Clayton, Victoria, Australia.
Department of Molecular and Translational Sciences, Monash University, Clayton, Victoria, Australia.
Andrology. 2020 Sep;8(5):1456-1470. doi: 10.1111/andr.12823. Epub 2020 Jun 12.
Snail transcription factors mediate key cellular transitions in many developmental processes, including spermatogenesis, and their production can be regulated by TGF-β superfamily signalling. SNAI1 and SNAI2 support many cancers of epithelial origin. Their functional relevance and potential regulation by TGF-β superfamily ligands in germ cell neoplasia are unknown.
SNAI1, SNAI2 and importin 5 (IPO5; nuclear transporter that selectively mediates BMP signalling) cellular localization was examined in fixed normal adult human and/or neoplastic testes using in situ hybridization and/or immunohistochemistry. SNAI1 and SNAI2 functions were assessed using the well-characterized human seminoma cell line, TCam-2. Cell migration, adhesion/proliferation and survival were measured by scratch assay, xCELLigence and flow cytometry following siRNA-induced reduction of SNAI1 and SNAI2 in TCam-2 cells. The potential regulation of SNAI1 and SNAI2 in TCam-2 cells by TGF-β signalling ligands, activin A and BMP4 was evaluated following 48 hours culture, including with siRNA regulation of IPO5 to selectively restrict BMP4 signalling.
In normal testes, SNAI1 transcript was identified in some spermatogonia and in spermatocytes, and SNAI2 protein localized to nuclei of spermatogonia, spermatocytes and round spermatids. In neoplastic testes, both SNAI1 and SNAI2 were detected in GCNIS and in seminoma cells. SNAI1 and SNAI2 reduction in TCam-2 cells by siRNAs significantly inhibited migration and survival, respectively. Exposure to BMP4, but not activin A, significantly increased SNAI2 (18-fold). IPO5 inhibition by siRNAs decreased BMP4-induced SNAI2 upregulation (5-fold). Additionally, SNAI2 reduction using siRNAs inhibited BMP4-induced TCam-2 cell survival.
This is the first evidence that SNAI1 and SNAI2 are involved in human spermatogenesis, with independent functions. These outcomes demonstrate that SNAI1 and SNAI2 inhibition leads to loss of migratory and viability capacities in seminoma cells. These findings show the potential for therapeutic treatments targeting SNAIL or BMP4 signalling for patients with metastatic testicular germ cell tumours.
蜗牛转录因子在许多发育过程中调节关键的细胞转化,包括精子发生,其产生可受 TGF-β 超家族信号的调节。SNAI1 和 SNAI2 支持许多上皮来源的癌症。它们在生殖细胞肿瘤中的功能相关性及其潜在的 TGF-β 超家族配体调节尚不清楚。
使用原位杂交和/或免疫组织化学检查固定的正常成人和/或肿瘤睾丸中 SNAI1、SNAI2 和进口蛋白 5(IPO5;选择性介导 BMP 信号的核转运蛋白)的细胞定位。使用经过充分表征的人精原细胞瘤细胞系 TCam-2 评估 SNAI1 和 SNAI2 的功能。在 TCam-2 细胞中用 siRNA 降低 SNAI1 和 SNAI2 后,通过划痕试验、xCELLigence 和流式细胞术测量细胞迁移、粘附/增殖和存活。评估 TGF-β 信号配体激活素 A 和 BMP4 对 TCam-2 细胞中 SNAI1 和 SNAI2 的潜在调节作用,包括用 siRNA 调节 IPO5 以选择性限制 BMP4 信号。
在正常睾丸中,SNAI1 转录本在一些精原细胞和精母细胞中被鉴定,SNAI2 蛋白定位于精原细胞、精母细胞和圆形精子细胞的核内。在肿瘤睾丸中,GCNIS 和精原细胞瘤细胞中均检测到 SNAI1 和 SNAI2。siRNA 降低 TCam-2 细胞中的 SNAI1 和 SNAI2 分别显著抑制迁移和存活。BMP4 暴露(而非激活素 A)显著增加 SNAI2(18 倍)。siRNA 抑制 IPO5 减少 BMP4 诱导的 SNAI2 上调(5 倍)。此外,siRNA 降低 SNAI2 抑制 BMP4 诱导的 TCam-2 细胞存活。
这是第一个证明 SNAI1 和 SNAI2 参与人类精子发生的证据,具有独立的功能。这些结果表明,SNAI1 和 SNAI2 抑制导致精原细胞瘤细胞丧失迁移和存活能力。这些发现表明针对 SNAIL 或 BMP4 信号的治疗方法具有治疗转移性睾丸生殖细胞肿瘤患者的潜力。
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