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A simple and sensitive enzymatic method for cholesterol quantification in macrophages and foam cells

机译:一种简单而灵敏的酶法测定巨噬细胞和泡沫细胞中的胆固醇

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摘要

A precise and sensitive method for measuring cellular free and esterified cholesterol is required in order to perform studies of macrophage cholesterol loading, metabolism, storage, and efflux. Until now, the use of an enzymatic cholesterol assay, commonly used for aqueous phase plasma cholesterol assays, has not been optimized for use with solid phase samples such as cells, due to inefficient solubilization of total cholesterol in enzyme compatible solvents. We present an efficient solubilization protocol compatible with an enzymatic cholesterol assay that does not require chemical saponification or chromatographic separation. Another issue with enzyme compatible solvents is the presence of endogenous peroxides that interfere with the enzymatic cholesterol assay. We overcame this obstacle by pretreatment of the reaction solution with the enzyme catalase, which consumed endogenous peroxides resulting in reduced background and increased sensitivity in our method. Finally, we demonstrated that this method for cholesterol quantification in macrophages yields results that are comparable to those measured by stable isotope dilution gas chromatography with mass spectrometry detection. In conclusion, we describe a sensitive, simple, and high-throughput enzymatic method to quantify cholesterol in complex matrices such as cells.
机译:为了进行巨噬细胞胆固醇负载,代谢,储存和外排的研究,需要一种精确而灵敏的方法来测量细胞中游离和酯化的胆固醇。迄今为止,由于总胆固醇在酶相容性溶剂中的溶解度较低,因此尚未将用于水相血浆胆固醇测定的酶促胆固醇测定法优化用于固相样品(如细胞)。我们提出了与酶促胆固醇测定兼容的有效增溶方案,不需要化学皂化或色谱分离。与酶相容的溶剂的另一个问题是内源性过氧化物的存在会干扰酶促胆固醇的测定。我们通过用过氧化氢酶预处理反应溶液克服了这一障碍,过氧化氢酶消耗了内源性过氧化物,导致本发明方法的背景降低并提高了灵敏度。最后,我们证明了这种在巨噬细胞中进行胆固醇定量的方法所产生的结果与采用质谱检测的稳定同位素稀释气相色谱法测得的结果相当。总之,我们描述了一种灵敏,简单且高通量的酶促方法,用于定量测定复杂基质(例如细胞)中的胆固醇。

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