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大鼠和人体组织中多萜醇及磷酸多萜醇的分离、定量与分布

Separation, quantitation and distribution of dolichol and dolichyl phosphate in rat and human tissues.

作者信息

Eggens I, Chojnacki T, Kenne L, Dallner G

出版信息

Biochim Biophys Acta. 1983 May 16;751(3):355-68. doi: 10.1016/0005-2760(83)90294-1.

Abstract

Two procedures for quantitative determination of dolichol were studied and these were applied to analyze tissue and subcellular distribution. In the first procedure the dolichols were oxidized with Cr2O3 and reduced with NaB3H4. The radioactivity in the individual dolichols was measured using reversed-phase thin-layer chromatography. In the second procedure, dolichols were analyzed by high-pressure liquid chromatography. For determination of dolichyl phosphates the lipid extract was subjected to acid and alkaline hydrolysis, and after hydrolysis with acid phosphatase the distribution was determined by high-pressure liquid chromatography. Recovery was monitored by the addition of dolichol D15 and D23 phosphate to the homogenate. Rat spleen had the highest dolichol content (114 micrograms/g) followed by lower content in rat liver and brain. The distribution pattern was similar in all organs, with 18 and 19 isoprene residues as dominating components. Human organs contain considerably higher concentrations of dolichol, with the 19 and 20 isoprene residues as the main components. In rat liver, outer mitochondrial and Golgi membranes, lysosomes and plasma membranes contain considerable amounts of dolichol. A drastic increase in dolichol content was observed in rat liver hyperplastic nodules while human liver cirrhosis and hepatocarcinoma showed a marked decrease in dolichol. In the latter case, the distribution pattern was also changed. Of the total amount of dolichol present in the tissues, 2% was phosphorylated in human liver, 10% in human testis and 18% in rat liver. In rat liver mitochondria and in microsomes 4 and 31%, respectively, of the polyprenols were in activated form. The results demonstrated that dolichyl phosphate and dolichol concentrations were regulated by different mechanisms and that the two forms possessed an independent distribution.

摘要

研究了两种定量测定多萜醇的方法,并将其应用于分析组织和亚细胞分布。在第一种方法中,多萜醇用Cr2O3氧化,并用NaB3H4还原。使用反相薄层色谱法测量各个多萜醇中的放射性。在第二种方法中,通过高压液相色谱法分析多萜醇。为了测定多萜醇磷酸酯,脂质提取物先进行酸水解和碱水解,然后用酸性磷酸酶水解后,通过高压液相色谱法测定其分布。通过向匀浆中添加多萜醇D15和D23磷酸酯来监测回收率。大鼠脾脏的多萜醇含量最高(114微克/克),其次是大鼠肝脏和大脑中的含量较低。所有器官中的分布模式相似,以18和19个异戊二烯残基为主要成分。人体器官中多萜醇的浓度要高得多,以19和20个异戊二烯残基为主要成分。在大鼠肝脏中,线粒体外膜、高尔基体膜、溶酶体和质膜含有大量的多萜醇。在大鼠肝脏增生性结节中观察到多萜醇含量急剧增加,而人类肝硬化和肝癌中多萜醇含量显著降低。在后一种情况下,分布模式也发生了变化。在组织中存在的多萜醇总量中,人类肝脏中2%被磷酸化,人类睾丸中10%被磷酸化,大鼠肝脏中18%被磷酸化。在大鼠肝脏线粒体和微粒体中,分别有4%和31%的聚戊烯醇处于活化形式。结果表明,多萜醇磷酸酯和多萜醇的浓度受不同机制调节,且这两种形式具有独立的分布。

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