首页> 外文期刊>Journal of Lipid Research >Preparation and incorporation of probe-labeled apoA-I for fluorescence resonance energy transfer studies of rHDL.
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Preparation and incorporation of probe-labeled apoA-I for fluorescence resonance energy transfer studies of rHDL.

机译:探针标记的apoA-I的制备和掺入,用于rHDL的荧光共振能量转移研究。

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摘要

Apolipoprotein A-I (apoA-I), the major constituent of HDL, plays an essential role in regulating cholesterol metabolism, acting as the physiological activator of lecithin: cholesterol acyltransferase, which converts cholesterol to cholesterol ester. Thiol-reactive fluorescent probes attached to cysteine-containing apoA-I mutants are currently being used to investigate the "LCAT active" conformation of lipid-bound apoA-I. Herein, we report new methodologies allowing rapid expression, fluorescent labeling, and recombinant HDL (rHDL) preparation for use in apoA-I in fluorescence resonance energy transfer (FRET) studies. Cysteine-containing mutant forms of human apoA-I were cloned into the pTYB12 vector containing a T7 promoter, a modified self-splicing protein element (intein), and a small affinity tag [chitin binding domain (CBD)]. The fusion proteins were expressed in Escherichia coli, isolated from cell lysates, and bound to a chitin-affinity column. Release of mature human apoA-I was initiated by the addition of DTT, which induced self-cleavage at the COOH terminus of the intein - CBD fusion protein. ApoA-I was further purified by Q-sepharose and then used for fluorescent probe labeling. Discoidal rHDL were then prepared with donor and/or acceptor labeled apoA-I and characterized with respect to their size, composition and ability to activate LCAT.
机译:载脂蛋白A-I(apoA-I)是HDL的主要成分,在调节胆固醇代谢中起着至关重要的作用,它是卵磷脂的生理活化剂:胆固醇酰基转移酶,可将胆固醇转化为胆固醇酯。与含半胱氨酸的apoA-I突变体连接的硫醇反应性荧光探针目前正用于研究脂质结合apoA-I的“ LCAT活性”构象。在这里,我们报告了新的方法,允许快速表达,荧光标记和重组HDL(rHDL)制备用于apoA-I在荧光共振能量转移(FRET)研究中。将含半胱氨酸的人类apoA-I突变体克隆到pTYB12载体中,该载体包含T7启动子,修饰的自剪接蛋白元件(内含肽)和小的亲和标签[几丁质结合域(CBD)]。融合蛋白在大肠杆菌中表达,从细胞裂解物中分离出来,并与几丁质亲和柱结合。通过添加DTT引发成熟人apoA-I的释放,DTT诱导内含蛋白-CBD融合蛋白COOH末端的自我切割。 ApoA-I通过Q-琼脂糖进一步纯化,然后用于荧光探针标记。然后用供体和/或受体标记的apoA-1制备盘状rHDL,并对其大小,组成和激活LCAT的能力进行表征。

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