白细胞介素-4 启动子内单核苷酸多态性对哮喘患者阿司匹林不耐受的影响及白细胞介素-4 启动子活性。

Effect of single nucleotide polymorphisms within the interleukin-4 promoter on aspirin intolerance in asthmatics and interleukin-4 promoter activity.

机构信息

Division of Molecular and Life Sciences, College of Science and Technology, Hanyang University, Sangrok Ku, Ansan, Gyeonggi-Do, Korea.

出版信息

Pharmacogenet Genomics. 2010 Dec;20(12):748-58. doi: 10.1097/FPC.0b013e3283402155.

DOI:10.1097/FPC.0b013e3283402155

PMID:20921925

Abstract

OBJECTIVE

Aspirin affects interleukin-4 (IL-4) synthesis; however, the genetic role of IL-4 has not been evaluated in asthmatics with aspirin hypersensitivity. The objective of the study was to examine the influence of single nucleotide polymorphisms (SNPs) in IL-4 gene on aspirin hypersensitivity in asthmatics at the genetic and molecular levels.

METHODS

Aspirin-intolerant (AIA, n=103) and aspirin-tolerant asthmatics (n=270) were genotyped and functional promoter assays were performed.

RESULTS

Of 15 SNPs tested, seven (-589T>C (rs2243250) in promoter, -33T>C (rs2070874) in the 5'-untranslated region, +4047A>G (rs2243266), +4144C>G (rs2243267), +4221C>A (rs2243268), +4367G>A (rs2243270), and +5090A>G (rs2243274) in introns) were significantly associated with AIA risk. The frequency of the rare allele (C) of -589T>C was higher in the AIA group than in the aspirin-tolerant asthmatic group (P=0.016), and a gene dose-dependent decline in forced expiratory volume in 1 s was noted after an aspirin challenge (P=0.0009). Aspirin unregulated IL-4 mRNA production in Jurkat T and K562 leukemia cells. A reporter plasmid assay revealed that aspirin augmented IL-4 promoter transactivation with the -589T>C C and -33T>C C alleles, compared with that bearing the -589T>C T and -33T>C T alleles. Further, electrophoretic mobility shift assay showed the formation of nuclear complexes with -33T>C and -589T>C allele-containing probes; this was augmented by aspirin. The complexes formed with the -33T>C and -589T>C probes were shifted by treatment with anti-CCAAT-enhancer-binding proteins β and anti-nuclear factor of activated T-cells antibodies, respectively, indicating the inclusion of these transcription factors.

CONCLUSION

Aspirin may regulate IL4 expression in an allele-specific manner by altering the availability of transcription factors to the key regulatory elements in the IL4 promoter, leading to aspirin hypersensitivity.

摘要

目的

阿司匹林会影响白细胞介素-4（IL-4）的合成；然而，IL-4 的遗传作用在阿司匹林过敏的哮喘患者中尚未得到评估。本研究的目的是从遗传和分子水平上研究白细胞介素-4 基因的单核苷酸多态性（SNP）对阿司匹林过敏的哮喘患者的影响。

方法

对不耐受阿司匹林的哮喘患者（AIA，n=103）和耐受阿司匹林的哮喘患者（n=270）进行基因分型，并进行功能性启动子检测。

结果

在检测的 15 个 SNP 中，有 7 个 SNP（启动子中的-589T>C（rs2243250）、5'-非翻译区中的-33T>C（rs2070874）、+4047A>G（rs2243266）、+4144C>G（rs2243267）、+4221C>A（rs2243268）、+4367G>A（rs2243270）和内含子中的+5090A>G（rs2243274））与 AIA 风险显著相关。-589T>C 的罕见等位基因（C）在 AIA 组中的频率高于阿司匹林耐受的哮喘组（P=0.016），并且在阿司匹林挑战后观察到 1 秒用力呼气量的基因剂量依赖性下降（P=0.0009）。阿司匹林可上调 Jurkat T 和 K562 白血病细胞中 IL-4 的 mRNA 产生。报告质粒试验表明，与携带-589T>C T 和-33T>C T 等位基因的对照相比，阿司匹林增强了 IL-4 启动子的转录激活，-589T>C C 和-33T>C C 等位基因。此外，电泳迁移率变动分析显示，含有-33T>C 和-589T>C 等位基因的探针形成核复合物，阿司匹林可增强其形成。用抗 CCAAT 增强子结合蛋白β和抗激活 T 细胞核因子抗体处理后，用-33T>C 和-589T>C 探针形成的复合物发生移动，表明这些转录因子的参与。