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一种新型的活体测量外周巨噬细胞胆固醇质量通量的方法。

Novel in vivo method for measuring cholesterol mass flux in peripheral macrophages.

机构信息

Division of Gastroenterology, Hepatology and Nutrition, The Children's Hospital of Philadelphia, Philadelphia, PA, USA.

出版信息

Arterioscler Thromb Vasc Biol. 2011 Dec;31(12):2865-71. doi: 10.1161/ATVBAHA.111.236406. Epub 2011 Sep 22.

Abstract

OBJECTIVE

Reverse cholesterol transport is the process by which excess cholesterol is removed from peripheral tissue by HDL and delivered to the liver for excretion. Presently, methods of measuring in vivo reverse cholesterol transport do so by monitoring the appearance in the feces of labeled cholesterol that originated from peripheral macrophage foam cells. These methods do not account for changes in macrophage cholesterol mass. We have developed an in vivo assay to measure cholesterol mass changes in atherosclerotic foam cells.

METHODS AND RESULTS

Macrophages are entrapped in semipermeable (pore size 0.2 μm) hollow fibers and surgically implanted into the peritoneum of recipient mice. The fibers are removed from the peritoneum 24 hours after implantation. This method allows the complete recovery of the macrophages for quantification of changes in cholesterol mass and cellular protein. In wild-type mice we measured a significant reduction in total cell cholesterol (TC) when hollow fibers containing cholesterol-enriched macrophage cells were implanted (TC before implantation=105±18 μg/mg cell protein, TC 24 hours after implantation=60±16 μg/mg protein). Additionally, there was an increase in cholesterol content when hollow fibers containing cholesterol-normal macrophages were implanted in an atherogenic mouse model (LDLr/apobec dko) compared to a wild-type mouse (initial TC content=57±24 μg/mg protein, TC 24 hours after implantation: wild-type mice=52±10 μg/mg protein; LDLr/apobec dko mice=118±27 μg/mg protein).

CONCLUSIONS

This assay can quantify in vivo both cholesterol mass accumulation, and reduction, in macrophages. This method permits quantitative analysis of the progression and regression of foam cells.

摘要

目的

胆固醇逆向转运是指高密度脂蛋白(HDL)将外周组织中多余的胆固醇运走,并将其运送到肝脏进行排泄的过程。目前,测量体内胆固醇逆向转运的方法是通过监测源自外周巨噬细胞泡沫细胞的标记胆固醇在粪便中的出现来进行。这些方法没有考虑到巨噬细胞胆固醇质量的变化。我们已经开发了一种体内测定法来测量动脉粥样硬化泡沫细胞中胆固醇质量的变化。

方法和结果

巨噬细胞被包裹在半透性(孔径 0.2μm)空心纤维中,并通过手术植入到受体小鼠的腹膜中。植入后 24 小时从腹膜中取出纤维。这种方法允许对巨噬细胞进行完整回收,以定量测量胆固醇质量和细胞蛋白的变化。在野生型小鼠中,我们测量到含有富含胆固醇的巨噬细胞的空心纤维植入后总细胞胆固醇(TC)显著减少(植入前 TC=105±18μg/mg 细胞蛋白,植入后 24 小时 TC=60±16μg/mg 蛋白)。此外,在动脉粥样硬化小鼠模型(LDLr/apobec dko)中,当植入含有胆固醇正常的巨噬细胞的空心纤维时,胆固醇含量增加,与野生型小鼠相比(初始 TC 含量=57±24μg/mg 蛋白,植入后 24 小时 TC:野生型小鼠=52±10μg/mg 蛋白;LDLr/apobec dko 小鼠=118±27μg/mg 蛋白)。

结论

该测定法可定量测量体内巨噬细胞中胆固醇质量的积累和减少。这种方法允许对泡沫细胞的进展和消退进行定量分析。

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