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用电免疫分析法测定人载脂蛋白C-II。体育锻炼前后的标准化及测定研究。

Determination of human apolipoprotein C-II by electroimmunoassay. Studies on standardization and determination before and after physical training.

作者信息

Jauhiainen M, Laitinen M, Penttilä I, Puhakainen E, Hietanen E

出版信息

Int J Biochem. 1983;15(4):501-6. doi: 10.1016/0020-711x(83)90123-4.

Abstract
  1. Human VLDL and HDL were fractionated by sequential ultracentrifugation until free of contaminant plasma proteins. 2. Column chromatofocusing method was used to isolate apolipoprotein C-II from apoVLDL and apo HDL. C-apoprotein peak was rechromatofocused and the second peak was the apo C-II (pI 4.7, homogeneous band on SDS slab gel). 3. New Zealand white rabbits were immunized with apo C-II. Antiserum gave a single precipitate are of identity between whole serum, apoVLDL, apoHDL and apo C-II. 4. Apo C-II concentration was measured by electroimmunoassay method. During standardization 1% Triton X-100 improved the rocket shapes and contours. Total delipidation did not affect the assay system and so the antigenic determinants of apo C-II are all available to antiserum. The lowest concentration of apo C-II possible to determine with this method was 70 ng/sample well. 5. There was no difference between the apo C-II values before (39.8 +/- 7.1 mg/l, n = 19) and after (41.6 +/- 6.4 mg/l, n = 19) moderate physical training among normolipemic subjects. 6. Specific immunoprecipitation technique was also used to determine apo C-II content in standard pool serum.
摘要
  1. 通过连续超速离心对人极低密度脂蛋白(VLDL)和高密度脂蛋白(HDL)进行分级分离,直至不含血浆蛋白污染物。2. 采用柱色谱聚焦法从极低密度脂蛋白(apoVLDL)和高密度脂蛋白(apo HDL)中分离载脂蛋白C-II。对C-载脂蛋白峰进行再次色谱聚焦,第二个峰即为载脂蛋白C-II(pI 4.7,在十二烷基硫酸钠平板凝胶上呈均一性条带)。3. 用载脂蛋白C-II免疫新西兰白兔。抗血清在全血清、极低密度脂蛋白、高密度脂蛋白和载脂蛋白C-II之间产生单一沉淀带。4. 采用电免疫分析法测定载脂蛋白C-II浓度。在标准化过程中,1% Triton X-100改善了火箭形状和轮廓。完全脱脂不影响检测系统,因此载脂蛋白C-II的抗原决定簇均可与抗血清结合。用该方法能够测定的载脂蛋白C-II的最低浓度为70 ng/样品孔。5. 在血脂正常的受试者中,适度体育锻炼前(39.8±7.1 mg/l,n = 19)和锻炼后(41.6±6.4 mg/l,n = 19)的载脂蛋白C-II值无差异。6. 还采用特异性免疫沉淀技术测定标准混合血清中的载脂蛋白C-II含量。

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