MiRNA-103b Downregulates ITGB3 and Mediates Apoptosis in Ex Vivo Stored Human Platelets.

Neetu Dahiya, Chintamani Atreya
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引用次数: 4

Abstract

Background: Blood bank-stored human platelets are one of the life-saving transfusion products to prevent bleeding in multiple clinical settings. In ex vivo storage, platelets undergo apoptosis and it is highly desirable to prevent this process to preserve platelet quality. However, underlying mechanisms of apoptosis are not well understood in stored platelets. Integrin beta 3 (ITGB3) glycoprotein plays multiple roles in platelet physiological processes, and it was reported in other cell types that downregulation of ITGB3 induces apoptosis. Small noncoding regulatory RNAs known as microRNAs (miRNAs), some of which are abundant in platelets such as miR-103b that belong to miR-103 family of miRNAs, known to play key roles in platelet functions both in vivo and during storage; Cellular miR-103 downregulates certain genes in other cell types and promotes apoptosis. However, whether miR-103b can target and downregulate ITGB3 in stored platelets and such miRNA regulation promotes apoptosis is not known. Here, we tested this working hypothesis.

Objective: Our objective of this study is to validate the abundance of miR-103b in stored platelets and identify whether ITGB3 is a target of miR-103b for the downregulation and this interaction promotes apoptosis.

Methods: RT-qPCR validation of miR-103b was performed in 11 donor samples at 3 different storage time points. In-silico analysis was performed to identify predicted targets of the miR-103b. The miRNA and messenger RNA interactions were confirmed using different biochemical approaches such as qRT-PCR, western blotting and, suppression of luciferase reporter gene expression by ectopic expression of miR-103b in HeLa cells. Final validation of the functional role of miR-103b in ITGB3 downregulation and resulting induction of apoptosis was assessed in stored platelets by FACS analysis following ectopic expression of miR-103b.

Results: Using the Target Scan Vert algorithm, we identified several integrin subunit-encoding mRNAs as potential targets of miR-103b. While ITGB3 and ITGB6 were found to have two targeting sites for miR-103b, since ITGB3 is known to play a role in apoptosis, we chose this for further validation in this study. Ectopic expression of miR-103b decreased the luciferase reporter activity in HeLa cells and decreased ITGB3 mRNA and protein levels in platelets, concomitant with an increase in apoptosis.

Conclusion: The results demonstrate that in stored platelets, miR-103b is highly expressed and can interact with and downregulate ITGB3 and promote apoptosis in stored platelets.

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MiRNA-103b下调ITGB3并介导体外储存人血小板凋亡
背景:血库储存的人血小板是多种临床环境中预防出血的救命输血产品之一。在离体储存中,血小板会发生凋亡,为了保持血小板的质量,防止这一过程是非常必要的。然而,在储存的血小板中,细胞凋亡的潜在机制尚不清楚。整合素β 3 (Integrin beta 3, ITGB3)糖蛋白在血小板生理过程中发挥多重作用,有报道称在其他细胞类型中ITGB3下调可诱导细胞凋亡。小的非编码调节rna被称为microRNAs (miRNAs),其中一些在血小板中丰富,如miR-103b,属于miR-103 miRNAs家族,已知在体内和储存过程中对血小板功能起关键作用;细胞miR-103在其他细胞类型中下调某些基因并促进细胞凋亡。然而,miR-103b是否能够靶向并下调储存血小板中的ITGB3,以及这种miRNA调控是否促进细胞凋亡尚不清楚。在这里,我们检验了这个可行的假设。目的:我们本研究的目的是验证miR-103b在储存血小板中的丰度,并确定ITGB3是否是miR-103b下调的靶标,并通过这种相互作用促进细胞凋亡。方法:在3个不同的储存时间点对11个供体样本进行miR-103b的RT-qPCR验证。进行计算机分析以确定miR-103b的预测靶标。通过不同的生化方法,如qRT-PCR、western blotting和通过在HeLa细胞中异位表达miR-103b抑制荧光素酶报告基因的表达,证实了miRNA和信使RNA的相互作用。在异位表达miR-103b后,通过FACS分析在储存的血小板中评估miR-103b在ITGB3下调和诱导细胞凋亡中的功能作用。结果:使用Target Scan Vert算法,我们确定了几个整合素亚基编码mrna作为miR-103b的潜在靶标。虽然我们发现ITGB3和ITGB6有两个miR-103b的靶向位点,但由于ITGB3已知在细胞凋亡中起作用,我们在本研究中选择了ITGB3进行进一步验证。miR-103b的异位表达降低了HeLa细胞中荧光素酶报告细胞活性,降低了血小板中ITGB3 mRNA和蛋白水平,同时细胞凋亡增加。结论:结果表明,在储存血小板中,miR-103b高表达,可与ITGB3相互作用并下调ITGB3,促进储存血小板凋亡。
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