Batiste Maryann, Joy Bethany, Yee Cara K, Cho Luke, Christensen Ashley, Abed Ihab, Nguyen Kailey, Yanumula Anusri, Chang Hannah, Cho Evan D, Wang Wenjia, Chou Emily, Chang Esther H, Shyu Yennie L, Abram Alyssa, Alcaide Jessa, Zhou James, Gillespie Brittany, Senderovich Michelle, Cusick Gianne Almeida, Le Ai-Vy, Hoang Frank, Shi Yihui, Mohamed Eslam, Cusick John K
Department of Basic Science, College of Medicine, California Northstate University, Elk Grove, CA 95757, USA.
Masters of Pharmaceutical Sciences Department, College of Graduate Studies, California Northstate University, Elk Grove, CA 95757, USA.
Biomedicines. 2024 Nov 22;12(12):2667. doi: 10.3390/biomedicines12122667.
Receptor Expressed in Lymphoid Tissues (RELT) is a TNFRSF member that has two paralogs, RELL1 and RELL2; the three proteins are collectively referred to as RELT family members (RELTfms).
We sought to evaluate RELT expression in cancerous cells by using real-time PCR, western blotting, flow cytometry, and immunohistochemistry (IHC). The mechanism of RELT-induced cell death was assessed by western blotting, flow cytometry, luciferase assays, and morphology staining. RELT localization was detected through immunofluorescence and western blotting, and co-immunoprecipitation was used to test whether a mutated RELT interacts with the OXSR1 kinase.
RELT and RELL1 protein expression was significantly elevated in cell lines representing breast and lung cancer, whereas RELL2 protein expression was relatively consistent across different cell lines. The surface expression of RELT was highest in monocytes. IHC staining revealed increased RELT expression in malignant breast cancer biopsies compared to patient-matched benign tissue. RELTfm overexpression induced death in MDA-MB-231 (231) breast cancer cells, accompanied by increased phosphatidylserine externalization and Caspase-3/7 activation. The co-transfection of plasmids predicted to block the phosphorylation of RELT by the OXSR1 kinase did not abrogate RELT-induced apoptosis, indicating that the activation of p38 by RELT through the OXSR1 kinase is not required for RELT-induced cell death. Interestingly, nuclear localization of RELT was detected in 231 and HEK-293 cells.
These results demonstrate that RELT induces death in breast cancer cells through an apoptotic pathway that does not require OXSR1 phosphorylation and that RELT possesses the ability to translocate to the nucleus, a novel finding that warrants further investigation.
淋巴组织中表达的受体(RELT)是肿瘤坏死因子受体超家族(TNFRSF)的成员,有两个旁系同源物RELL1和RELL2;这三种蛋白统称为RELT家族成员(RELTfms)。
我们试图通过实时聚合酶链反应(PCR)、蛋白质免疫印迹法、流式细胞术和免疫组织化学(IHC)来评估癌细胞中RELT的表达。通过蛋白质免疫印迹法、流式细胞术、荧光素酶测定和形态学染色来评估RELT诱导细胞死亡的机制。通过免疫荧光和蛋白质免疫印迹法检测RELT的定位,并使用免疫共沉淀法来检测突变的RELT是否与OXSR1激酶相互作用。
在代表乳腺癌和肺癌的细胞系中,RELT和RELL1蛋白表达显著升高,而RELL2蛋白表达在不同细胞系中相对一致。RELT的表面表达在单核细胞中最高。免疫组织化学染色显示,与患者匹配的良性组织相比,恶性乳腺癌活检组织中RELT表达增加。RELTfm过表达诱导MDA-MB-231(231)乳腺癌细胞死亡,同时磷脂酰丝氨酸外化增加和半胱天冬酶-3/7激活。共转染预计可阻断OXSR1激酶对RELT磷酸化的质粒并未消除RELT诱导的细胞凋亡,这表明RELT通过OXSR1激酶激活p38并非RELT诱导细胞死亡所必需。有趣的是,在231和HEK-293细胞中检测到RELT的核定位。
这些结果表明,RELT通过一条不需要OXSR1磷酸化的凋亡途径诱导乳腺癌细胞死亡,并且RELT具有转运至细胞核的能力,这一新颖发现值得进一步研究。
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