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用人血浆载脂蛋白C-II的放射免疫测定法进行免疫化学研究。

Immunochemistry of human plasma apolipoprotein C-II as studied by radioimmunoassay.

作者信息

Barr S I, Kottke B A, Chang J Y, Mao S J

出版信息

Biochim Biophys Acta. 1981 Feb 23;663(2):491-505. doi: 10.1016/0005-2760(81)90177-6.

DOI:10.1016/0005-2760(81)90177-6
PMID:7213782
Abstract

The immunoreactivity of human plasma apolipoprotein C-II was investigated using a specific radioimmunoassay. In whole plasma, the mean value quantitated was 2.21 +/- 0.415 mg/dl, while in delipidated plasma, a mean value of 3.84 +/- 1.186 mg/dl was obtained, suggesting that the antigenic sites of the apolipoprotein were not fully detected in unmodified plasma by our antibody preparation. Two detergents, Tween-20 and Triton X-100, were studied to determine if they could enhance the immunoreactivity of apolipoprotein C-II in whole plasma. At concentrations of 0.012-0.06%, Tween-20 markedly increased the immunoreactivity of whole plasma, but not of delipidated plasma, indicating that antigenic sites of plasma apolipoprotein C-II has been exposed by Tween-20. In contrast, Triton X-100 had no effect on the immunoreactivity of whole plasma apolipoprotein C-II. A radioimmunoassay conducted in the presence of 0.06% Tween-20, resulted in a mean value in whole plasma (3.39 +/- 1.11 mg/dl) that was not significantly different from that obtained when the assay was done on delipidated samples. The immunoreactivity of VLDL apolipoprotein C-II was also drastically enhanced following lipolysis by bovine milk lipoprotein lipase, supporting the hypothesis that antigenic sites are masked by the lipids. Finally, the mechanism responsible for the effect of Tween-20 on apolipoprotein C-II immunoreactivity was investigated. The results obtained from circular dichroism and ultracentrifugation suggest that the detergent may dissociate the apolipoprotein from lipoprotein particles, thus fully exposing the antigenic sites for reaction with antibodies.

摘要

使用特异性放射免疫分析法研究了人血浆载脂蛋白C-II的免疫反应性。在全血中,定量的平均值为2.21±0.415mg/dl,而在脱脂血浆中,平均值为3.84±1.186mg/dl,这表明我们制备的抗体在未修饰的血浆中未完全检测到载脂蛋白的抗原位点。研究了两种去污剂吐温-20和曲拉通X-100,以确定它们是否能增强全血中载脂蛋白C-II的免疫反应性。在0.012%-0.06%的浓度下,吐温-20显著提高了全血的免疫反应性,但对脱脂血浆没有影响,这表明血浆载脂蛋白C-II的抗原位点已被吐温-20暴露。相比之下,曲拉通X-100对全血载脂蛋白C-II的免疫反应性没有影响。在0.06%吐温-20存在下进行的放射免疫分析,全血中的平均值(3.39±1.11mg/dl)与对脱脂样品进行分析时得到的值没有显著差异。牛乳脂蛋白脂肪酶脂解后,极低密度脂蛋白载脂蛋白C-II的免疫反应性也显著增强,支持了抗原位点被脂质掩盖的假说。最后,研究了吐温-20对载脂蛋白C-II免疫反应性影响的机制。圆二色性和超速离心得到的结果表明,去污剂可能使载脂蛋白与脂蛋白颗粒解离,从而充分暴露抗原位点以与抗体反应。

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Association between apolipoproteins A-I and A-II as evidenced by immunochemical approach.免疫化学方法证实的载脂蛋白A-I与A-II之间的关联。
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Purification, cloning and nucleotide sequence determination of cynomolgus monkey apolipoprotein C-II: comparison to the human sequence.食蟹猴载脂蛋白C-II的纯化、克隆及核苷酸序列测定:与人类序列的比较
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Am J Hum Genet. 1991 Dec;49(6):1155-66.