一种测定家族性高胆固醇血症中功能性低密度脂蛋白受体活性的新方法：CD3/CD28 检测法在淋巴细胞中的应用。

A novel method for determining functional LDL receptor activity in familial hypercholesterolemia: application of the CD3/CD28 assay in lymphocytes.

作者信息

Tada Hayato, Kawashiri Masa-aki, Noguchi Tohru, Mori Mika, Tsuchida Masayuki, Takata Mutsuko, Nohara Atsushi, Inazu Akihiro, Kobayashi Junji, Yachie Akihiro, Mabuchi Hiroshi, Yamagishi Masakazu

机构信息

Division of Cardiovascular Medicine, Department of Internal Medicine, Graduate School of Medical Science, Kanazawa University, Kanazawa, Japan.

出版信息

Clin Chim Acta. 2009 Feb;400(1-2):42-7. doi: 10.1016/j.cca.2008.10.010. Epub 2008 Oct 26.

DOI:10.1016/j.cca.2008.10.010

PMID:19013141

Abstract

BACKGROUND

The objective of this study was to develop a new and simple method for measuring low-density lipoprotein receptor (LDLR) activity using peripheral lymphocytes enabling us to clinically diagnose familial hypercholesterolemia (FH) and ascertain the involved mutations (such as K790X mutation), that might not be clearly detected in the conventional method.

METHODS

Our method comprised the following 2 features: first, we used anti-CD3/CD28 beads to stimulate T-lymphocytes to obtain a uniform fraction of lymphocytes and maximum up-regulation of LDLR. Second, we excluded the possibility of overestimation of lymphocyte signals bound only to its surface, by adding heparin to the cultured lymphocytes used for the LDLR assay.

RESULTS

Based on the genetic mutation, the FH subjects were divided into 2 groups, K790X, (n=20) and P664L, (n=5), and their LDLR activities was measured by this method, which was found to be 55.3+/-8.9% and 63.9+/-13.8%, respectively, of that of the control group (n=15). In comparison, the LDLR activity was 86.1+/-11.6% (K790X) and 73.3+/-6.3% (P664L) of that of the control group when measured by the conventional method, indicating that impairment of LDLR function in FH K790X subjects was much more clearly differentiated with our method than with the conventional method (paired t-test, p<0.0001). The levels of LDLR expression also showed similar tendencies, that is, 89.4+/-13.2% (K790X) and 76.9+/-17.4% (P664L) of that of the control group when measured by the conventional method, and 78.1+/-9.7% (K790X) and 70.3+/-26.5% (P664L) when measured by our new method. In addition, we confirmed that there was little influence of statin treatment on LDLR activity among the study subjects when our method was used.

CONCLUSION

These results demonstrate that our new method is applicable for measuring LDLR activity, even in subjects with an internally defective allele, and that T-lymphocytes of the FH K790X mutation possess characteristics of that allele.

摘要

背景

本研究的目的是开发一种新的、简单的方法，利用外周淋巴细胞测量低密度脂蛋白受体（LDLR）活性，使我们能够临床诊断家族性高胆固醇血症（FH）并确定相关突变（如K790X突变），而这些突变在传统方法中可能无法被清晰检测到。

方法

我们的方法包括以下两个特点：第一，我们使用抗CD3/CD28磁珠刺激T淋巴细胞，以获得均匀的淋巴细胞组分并使LDLR最大程度上调。第二，通过向用于LDLR检测的培养淋巴细胞中添加肝素，我们排除了仅与淋巴细胞表面结合的信号被高估的可能性。

结果

根据基因突变情况，FH受试者被分为两组，K790X组（n = 20）和P664L组（n = 5），并用此方法测量他们的LDLR活性，发现分别为对照组（n = 15）的55.3±8.9%和63.9±13.8%。相比之下，用传统方法测量时，K790X组和P664L组的LDLR活性分别为对照组的86.1±11.6%和73.3±6.3%，这表明与传统方法相比，我们的方法能更清晰地区分FH K790X受试者的LDLR功能受损情况（配对t检验，p < 0.0001）。LDLR表达水平也呈现类似趋势，即传统方法测量时，K790X组和P664L组分别为对照组的89.4±13.2%和76.9±17.4%，而用我们的新方法测量时分别为78.1±9.7%和70.3±26.5%。此外，我们证实，当使用我们的方法时，他汀类药物治疗对研究受试者的LDLR活性影响很小。