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基于单克隆抗体免疫测定法对血浆亚组分和细胞培养基中胆固醇酯转运蛋白进行低水平定量分析。

Low level quantification of cholesteryl ester transfer protein in plasma subfractions and cell culture media by monoclonal antibody-based immunoassay.

作者信息

Clark R W, Moberly J B, Bamberger M J

机构信息

Department of Cardiovascular and Metabolic Diseases, Pfizer, Inc., Groton, CT 06340, USA.

出版信息

J Lipid Res. 1995 Apr;36(4):876-89.

PMID:7639849
Abstract

Sensitive immunoradiometric (IRMA) and ELISA assays for cholesteryl ester transfer protein (CETP) have been developed using two different monoclonal antibodies (MAbs). The MAbs were prepared against human plasma CETP and demonstrated specificity by their inhibition of cholesteryl ester transfer activity and by immunoblots of crude plasma fractions and whole media from transfected CHO cells. For these sandwich-type assays, one MAb, 2F8, is used for capture, and the second MAb, 2E7, is iodinated (IRMA) or conjugated with alkaline phosphatase (ELISA) and used for detection. Both assays are linear and provide sensitivities much greater than previously reported. The IRMA allows for the accurate quantification of CETP in the range of 0.5-20 ng/assay (5-200 ng/ml), the ELISA 0.05-5 ng/assay (0.5-50 ng/ml). Using the IRMA, the mean plasma CETP concentration in 44 normolipidemic individuals was determined to be 2.10 +/- 0.36 micrograms/ml; 2.05 +/- 0.33 for males (n = 25) and 2.16 +/- 0.40 for females (n = 19). Values ranged from 1.28 to 2.97 micrograms/ml and CETP mass correlated well with cholesteryl ester transfer activity (r = 0.913, n = 23). The distribution of CETP in human plasma was examined both by gel permeation fast protein liquid chromatography (FPLC) and by native gel electrophoresis. For FPLC using agarose resins, a low ionic strength, isotonic buffer system resulted in near total recoveries of CETP, and demonstrated a peak for CETP mass centered at molecular masses of 150 to 180 kilodaltons, larger than that for free monomeric CETP. Native acrylamide gel electrophoresis of plasma from six individuals, followed by 2F8/2E7 sandwich immunoblotting, showed CETP migrating within a size range of 170-220 kilodaltons. This result is consistent with suggestions that plasma CETP is associated with small-sized HDL. Agarose gel electrophoresis showed plasma CETP, as well as purified recombinant CETP, to be prebeta migrating. For determining the concentration of CETP in the media of cultured HepG2 cells, advantage was taken of the high sensitivity of the ELISA. CETP levels were found to increase linearly over the 100-h culture period, reaching 8.0 +/- 0.4 ng/ml (18.0 +/- 1.3 ng/mg cell protein). These sensitive, direct immunoassays for CETP mass should be valuable aids for examining the behavior of CETP in plasma and other complex systems, as well as for studying the synthesis and secretion of CETP by different cells and tissues.

摘要

利用两种不同的单克隆抗体(MAb)开发了用于胆固醇酯转运蛋白(CETP)的灵敏免疫放射分析(IRMA)和酶联免疫吸附测定(ELISA)方法。这些单克隆抗体是针对人血浆CETP制备的,通过抑制胆固醇酯转运活性以及对来自转染CHO细胞的粗血浆组分和全培养基进行免疫印迹来证明其特异性。对于这些夹心型测定,一种单克隆抗体2F8用于捕获,第二种单克隆抗体2E7进行碘化(IRMA)或与碱性磷酸酶偶联(ELISA)并用于检测。两种测定均呈线性,且灵敏度远高于先前报道的水平。IRMA能够在0.5 - 20 ng/测定(5 - 200 ng/ml)范围内准确定量CETP,ELISA为0.05 - 5 ng/测定(0.5 - 50 ng/ml)。使用IRMA测定,44名血脂正常个体的平均血浆CETP浓度测定为2.10±0.36μg/ml;男性(n = 25)为2.05±0.33,女性(n = 19)为2.16±0.40。值范围为1.28至2.97μg/ml,CETP质量与胆固醇酯转运活性相关性良好(r = 0.913,n = 23)。通过凝胶渗透快速蛋白质液相色谱(FPLC)和天然凝胶电泳检测了CETP在人血浆中的分布。对于使用琼脂糖树脂的FPLC,低离子强度等渗缓冲系统可使CETP几乎完全回收,并显示CETP质量峰集中在150至180千道尔顿的分子量处,大于游离单体CETP的分子量。对6名个体的血浆进行天然丙烯酰胺凝胶电泳,随后进行2F8/2E7夹心免疫印迹,显示CETP在170 - 220千道尔顿的大小范围内迁移。该结果与血浆CETP与小尺寸高密度脂蛋白相关的推测一致。琼脂糖凝胶电泳显示血浆CETP以及纯化的重组CETP呈前β迁移。为了测定培养的HepG2细胞培养基中CETP的浓度,利用了ELISA的高灵敏度。发现CETP水平在100小时培养期内呈线性增加,达到8.0±0.4 ng/ml(18.0±1.3 ng/mg细胞蛋白)。这些用于CETP质量的灵敏直接免疫测定对于研究CETP在血浆和其他复杂系统中的行为,以及研究不同细胞和组织中CETP的合成和分泌应该是有价值的辅助手段。

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