小鼠而非人类的ephrin-B2可被丝氨酸蛋白酶激肽释放酶-4有效切割:对人类前列腺癌异种移植模型的启示。
Murine, but not human, ephrin-B2 can be efficiently cleaved by the serine protease kallikrein-4: implications for xenograft models of human prostate cancer.
作者信息
Lisle J E, Mertens-Walker I, Stephens C R, Stansfield S H, Clements J A, Herington A C, Stephenson S-A
机构信息
Institute of Health and Biomedical Innovation and the Australian Prostate Cancer Research Centre-Queensland, Queensland University of Technology, Translational Research Institute, Woolloongabba 4102, QLD, Australia.
Institute of Health and Biomedical Innovation and the Australian Prostate Cancer Research Centre-Queensland, Queensland University of Technology, Translational Research Institute, Woolloongabba 4102, QLD, Australia.
出版信息
Exp Cell Res. 2015 Apr 10;333(1):136-46. doi: 10.1016/j.yexcr.2015.02.014. Epub 2015 Feb 24.
BACKGROUND
Ephrin-B2 is the sole physiologically-relevant ligand of the receptor tyrosine kinase EphB4, which is over-expressed in many epithelial cancers, including 66% of prostate cancers, and contributes to cancer cell survival, invasion and migration. Crucially, however, the cancer-promoting EphB4 signalling pathways are independent of interaction with its ligand ephrin-B2, as activation of ligand-dependent signalling causes tumour suppression. Ephrin-B2, however, is often found on the surface of endothelial cells of the tumour vasculature, where it can regulate angiogenesis to support tumour growth. Proteolytic cleavage of endothelial cell ephrin-B2 has previously been suggested as one mechanism whereby the interaction between tumour cell-expressed EphB4 and endothelial cell ephrin-B2 is regulated to support both cancer promotion and angiogenesis.
METHODS
An in silico approach was used to search accessible surfaces of 3D protein models for cleavage sites for the key prostate cancer serine protease, KLK4, and this identified murine ephrin-B2 as a potential KLK4 substrate. Mouse ephrin-B2 was then confirmed as a KLK4 substrate by in vitro incubation of recombinant mouse ephrin-B2 with active recombinant human KLK4. Cleavage products were visualised by SDS-PAGE, silver staining and Western blot and confirmed by N-terminal sequencing.
RESULTS
At low molar ratios, KLK4 cleaved murine ephrin-B2 but other prostate-specific KLK family members (KLK2 and KLK3/PSA) were less efficient, suggesting cleavage was KLK4-selective. The primary KLK4 cleavage site in murine ephrin-B2 was verified and shown to correspond to one of the in silico predicted sites between extracellular domain residues arginine 178 and asparagine 179. Surprisingly, the highly homologous human ephrin-B2 was poorly cleaved by KLK4 at these low molar ratios, likely due to the 3 amino acid differences at this primary cleavage site.
CONCLUSION
These data suggest that in in vivo mouse xenograft models, endogenous mouse ephrin-B2, but not human tumour ephrin-B2, may be a downstream target of cancer cell secreted human KLK4. This is a critical consideration when interpreting data from murine explants of human EphB4+/KLK4+ cancer cells, such as prostate cancer cells, where differential effects may be seen in mouse models as opposed to human clinical situations.
背景
Ephrin-B2是受体酪氨酸激酶EphB4唯一在生理上相关的配体,EphB4在许多上皮癌中过度表达,包括66%的前列腺癌,并有助于癌细胞的存活、侵袭和迁移。然而,至关重要的是,促进癌症的EphB4信号通路独立于与其配体Ephrin-B2的相互作用,因为配体依赖性信号的激活会导致肿瘤抑制。然而,Ephrin-B2经常出现在肿瘤脉管系统的内皮细胞表面,在那里它可以调节血管生成以支持肿瘤生长。先前有人提出内皮细胞Ephrin-B2的蛋白水解切割是一种机制,通过这种机制可以调节肿瘤细胞表达的EphB4与内皮细胞Ephrin-B2之间的相互作用,以支持癌症促进和血管生成。
方法
采用计算机模拟方法在3D蛋白质模型的可及表面搜索关键前列腺癌丝氨酸蛋白酶KLK4的切割位点,结果确定小鼠Ephrin-B2为潜在的KLK4底物。然后通过将重组小鼠Ephrin-B2与活性重组人KLK4进行体外孵育,证实小鼠Ephrin-B2是KLK4底物。通过SDS-PAGE、银染和蛋白质印迹对切割产物进行可视化,并通过N端测序进行确认。
结果
在低摩尔比下,KLK4可切割小鼠Ephrin-B2,但其他前列腺特异性KLK家族成员(KLK2和KLK3/PSA)效率较低,表明切割具有KLK4选择性。验证了小鼠Ephrin-B2中主要的KLK4切割位点,并显示其对应于细胞外结构域残基精氨酸178和天冬酰胺179之间计算机模拟预测的位点之一。令人惊讶的是,在这些低摩尔比下,高度同源的人Ephrin-B2被KLK4切割的效率很低,这可能是由于该主要切割位点存在3个氨基酸差异。
结论
这些数据表明,在体内小鼠异种移植模型中,内源性小鼠Ephrin-B2而非人肿瘤Ephrin-B2可能是癌细胞分泌的人KLK4的下游靶点。在解释来自人EphB4+/KLK4+癌细胞(如前列腺癌细胞)的小鼠外植体数据时,这是一个关键的考虑因素,在小鼠模型中可能会看到与人类临床情况不同的效应。
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