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Effect of apolipoproteins E and C-III on the interaction of chylomicrons with parenchymal and non-parenchymal cells from rat liver

机译:载脂蛋白E和C-III对乳糜微粒与大鼠肝实质细胞和非实质细胞相互作用的影响

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p[3H]Triacylglycerol-labelled chylomicrons were isolated from intestinal lymph, obtained from rats made hypolipidaemic by treatment with pharmacological amounts of 17 alpha-ethynyloestradiol. Oestrogen treatment results in a large reduction in the content of apolipoproteins (apo) E and C of lymph chylomicrons. Upon incubation in vitro with freshly isolated parenchymal and non-parenchymal cells the apo E-, apo C-poor chylomicrons became readily cell-associated. With increasing chylomicron concentrations this cell-association was saturable and half-maximal cell-association was achieved at about 0.55 mg of triacylglycerol/ml. The cell-association was time- and temperature-dependent. A more than 90% inhibition of the cell-association of the [3H]triacylglycerol moiety was observed with both parenchymal and non-parenchymal cells when pure apo C-III (12.6 micrograms/mg of triacylglycerol) was incorporated into the chylomicrons. These data indicate that apo E-, apo C-poor chylomicrons are bound to both parenchymal and non-parenchymal liver cells at a high-affinity site of limited capacity and that binding to this site is strongly inhibited by apo C-III. With apo C-III-enriched chylomicrons simultaneous determination of the cell-association of the 125I-apo C-III and the [3H]triacylglycerol moiety indicated that more 125I-apo C-III becomes associated to the cells than expected on the basis of [3H]triacylglycerol radioactivity measurements. It is suggested that upon cell-association of apo C-III its binding to the chylomicron particles is lost. Consequently the occupation of the cellular recognition site by apo C-III prevents further chylomicron binding and thus leads to a decrease of the cell-association level of the [3H]triacylglycerol moiety. Apo E enrichment of the chylomicrons led to an increased cell-association rate with parenchymal cells and to a marked increase of the cell-association level with non-parenchymal cells. The cell-association of the apo E radioactivity followed closely the [3H]triacylglycerol radioactivity, indicating that the particle-apo E complex is bound as a unity. The apo E effects were opposed by apo C-III. With apo E-, apo C-III-enriched chylomicrons more 125I-apo E became associated with the cells than could be expected on the basis of the [3H]triacylglycerol measurements. It is concluded that apo C-III can weaken the interaction of apo E with the chylomicrons leading to the cell-association of free apo E. It appears that subtle changes in the apo E and/or apo C-III content of chylomicrons can influence the interaction with both parenchymal and non-parenchymal liver cells.(ABSTRACT TRUNCATED AT 400 WORDS)/p
机译:从肠道淋巴液中分离出[pH] [3H]甘油酰乳糜微粒,该小肠淋巴瘤是通过药理学剂量的17α-乙炔雌二醇处理而成的低血脂症大鼠的肠淋巴液。雌激素治疗可导致淋巴乳糜微粒的载脂蛋白(apo)E和C含量大大降低。在与新鲜分离的实质细胞和非实质细胞体外温育后,载脂蛋白E-,载脂蛋白C-贫的乳糜微粒变得容易与细胞缔合。随着乳糜微粒浓度的增加,这种细胞缔合是可饱和的,并且在约0.55mg的三酰基甘油/ ml下达到了半最大的细胞缔合。细胞关联是时间和温度依赖性的。当将纯载脂蛋白C-III(12.6微克/毫克三酰基甘油)掺入乳糜微粒时,在实质细胞和非实质细胞中都观察到[3H]三酰基甘油部分的细胞缔合有90%以上的抑制作用。这些数据表明,载脂蛋白E-,载脂蛋白C-贫乏的乳糜微粒在能力有限的高亲和力部位与实质和非实质性肝细胞结合,并且与该部位的结合受到载脂蛋白C-III的强烈抑制。利用富含载脂蛋白C-III的乳糜微粒,同时测定125I-载脂蛋白C-III和[3H]三酰基甘油部分的细胞缔合,表明与细胞缔合的125I-载脂蛋白C-III的数量比预期的要多。 [3 H]三酰基甘油放射性测量。提示在载脂蛋白C-III与细胞缔合后,它与乳糜微粒的结合就消失了。因此,载脂蛋白C-III对细胞识别位点的占据阻止了进一步的乳糜微粒结合,从而导致[3H]三酰基甘油部分的细胞缔合水平降低。乳糜微粒的Apo E富集导致与实质细胞的细胞缔合速率增加,而与非实质细胞的细胞缔合水平显着提高。载脂蛋白E放射性的细胞缔合与[3H]三酰基甘油放射性密切相关,表明颗粒-载脂蛋白E复合物被结合为一个整体。 Apo C-III反对Apo E的作用。有了载脂蛋白E-,富含载脂蛋白C-III的乳糜微粒与细胞缔合的125I-载脂蛋白E变得比根据[3H]三酰基甘油的测量结果所预期的要多。结论是载脂蛋白C-III可减弱载脂蛋白E与乳糜微粒的相互作用,从而导致游离载脂蛋白E的细胞缔合。看来乳糜微粒的载脂蛋白E和/或载脂蛋白C-III含量的细微变化可影响与实质和非实质肝细胞的相互作用。(摘要截断为400字)

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