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Scalable production of biliverdin IXα by Escherichia coli

机译:大肠杆菌可大规模生产BiliverdinIXα

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摘要

BackgroundBiliverdin IXα is produced when heme undergoes reductive ring cleavage at the α-methene bridge catalyzed by heme oxygenase. It is subsequently reduced by biliverdin reductase to bilirubin IXα which is a potent endogenous antioxidant. Biliverdin IXα, through interaction with biliverdin reductase, also initiates signaling pathways leading to anti-inflammatory responses and suppression of cellular pro-inflammatory events. The use of biliverdin IXα as a cytoprotective therapeutic has been suggested, but its clinical development and use is currently limited by insufficient quantity, uncertain purity, and derivation from mammalian materials. To address these limitations, methods to produce, recover and purify biliverdin IXα from bacterial cultures of Escherichia coli were investigated and developed.
机译:背景当血红素在血红素加氧酶催化的α-亚甲基桥上进行还原性环裂解时,会产生BiliverdinIXα。随后通过胆绿素还原酶将其还原为有效的内源性抗氧化剂胆红素IXα。 BiliverdinIXα通过与biliverdin还原酶相互作用,还启动了导致抗炎反应和抑制细胞促炎事件的信号传导途径。已经提出了使用胆绿素IXα作为细胞保护性治疗剂的用途,但是其临床开发和使用目前受到数量不足,纯度不确定和源自哺乳动物材料的限制。为了解决这些局限性,研究和开发了从大肠杆菌细菌培养物中生产,回收和纯化比利韦丁IXα的方法。

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