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鸽单核细胞衍生巨噬细胞中脂蛋白细胞内运输的同步标记

Simultaneous labeling of lipoprotein intracellular trafficking in pigeon monocyte-derived macrophages.

作者信息

Jones N L

机构信息

Pathology Department, Bowman Gray School of Medicine, Wake Forest University, Winston-Salem, North Carolina 27157, USA.

出版信息

Am J Pathol. 1997 Mar;150(3):1113-24.

Abstract

Macrophage foam cell formation resulting from the accumulation of cholesterol and cholesterol esters derived from plasma lipoproteins is important for progression of atherosclerosis. Hypothetically, intracellular processing of lipoproteins that stimulate foam cell formation differs from processing of lipoproteins that do not. To test this, we examined simultaneous subcellular trafficking of lipoproteins in pigeon monocyte-derived macrophages. Pigeon beta-very-low-density lipoprotein (beta-VLDL), low-density lipoprotein (LDL), and acetylated low-density lipoprotein (Ac-LDL), differentially labeled with colloidal gold, were added in pairs to cells at 4 degrees C for 2 hours before uptake at 18 degrees C, 22 degrees C, or 37 degrees C for either 30 minutes or 2 hours. The colloidal gold distribution and percent co-labeling as observed by transmission electron microscopy were determined for organelles of the endocytic pathway. Incubations at 18 degrees C and 22 degrees C blocked lipoprotein trafficking to lysosomes. Incubation at 18 degrees C increased the percent distribution of lipoproteins in the endocytic pathway up to the early cisternal endosomes. Incubations at 22 degrees C resulted in a greater distribution of lipoproteins in the spherical late endosomes and late endosomal-prelysosomal tubular reticular compartment. The distribution in the endocytic pathway was a factor of time and temperature rather than lipoprotein type. The percentage of co-labeling of organelles for the three pairs of lipoproteins examined, Ac-LDL plus beta-VLDL, LDL plus beta-VLDL, and LDL plus Ac-LDL, was similar. Fewer noncoated and clathrin-coated pits and vesicles were co-labeled (average of 6%, maximum of 17%) than the rest of the endocytic pathway, early cisternal endosomes, spherical late endosomes, late endosomal-prelysosomal tubuloreticular compartment, and spherical lysosomes (average of 36%, maximum of 47%). The 36% of co-labeled later endocytic organelles contained an average of 58% of the labeled lipoproteins. This study suggests differential sorting does not occur for high-affinity uptake of lipoproteins.

摘要

由源自血浆脂蛋白的胆固醇和胆固醇酯积累导致的巨噬细胞泡沫细胞形成对动脉粥样硬化的进展很重要。据推测,刺激泡沫细胞形成的脂蛋白的细胞内加工与不刺激泡沫细胞形成的脂蛋白的加工不同。为了验证这一点,我们研究了鸽单核细胞衍生巨噬细胞中脂蛋白的同时亚细胞运输。用胶体金进行差异标记的鸽β-极低密度脂蛋白(β-VLDL)、低密度脂蛋白(LDL)和乙酰化低密度脂蛋白(Ac-LDL),在4℃下与细胞成对孵育2小时,然后在18℃、22℃或37℃下摄取30分钟或2小时。通过透射电子显微镜观察确定内吞途径细胞器的胶体金分布和共标记百分比。在18℃和22℃下孵育会阻止脂蛋白运输到溶酶体。在18℃下孵育会增加脂蛋白在内吞途径中直至早期池状内体的分布百分比。在22℃下孵育会导致脂蛋白在球形晚期内体和晚期内体 - 前溶酶体管状网状区室中分布更多。在内吞途径中的分布是时间和温度的函数,而不是脂蛋白类型的函数。所检测的三对脂蛋白(Ac-LDL加β-VLDL、LDL加β-VLDL和LDL加Ac-LDL)细胞器的共标记百分比相似。与内吞途径的其他部分(早期池状内体、球形晚期内体、晚期内体 - 前溶酶体管状网状区室和球形溶酶体)相比,被共标记的无包被和网格蛋白包被的小窝和囊泡较少(平均6%,最大17%)。36%的共标记晚期内吞细胞器平均含有58%的标记脂蛋白。这项研究表明,对于脂蛋白的高亲和力摄取不会发生差异分选。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e81b/1857901/227ca547b644/amjpathol00027-0332-a.jpg

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