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白细胞介素-13基因与白细胞介素-4基因的共表达,与其在人类5号染色体5q23 - 31细胞因子基因簇中的物理连锁相关。

Coexpression of the interleukin-13 and interleukin-4 genes correlates with their physical linkage in the cytokine gene cluster on human chromosome 5q23-31.

作者信息

Dolganov G, Bort S, Lovett M, Burr J, Schubert L, Short D, McGurn M, Gibson C, Lewis D B

机构信息

Genelabs Incorporated, Redwood City, CA USA.

出版信息

Blood. 1996 Apr 15;87(8):3316-26.

PMID:8605348
Abstract

Interleukin-13 (IL-13) and IL-4 are cytokines produced by T cells that are encoded by the q23-31 region of human chromosome 5. To investigate the regulation of IL-13 gene expression by T cells, we isolated and sequenced the human IL-13 gene, analyzed its 5'-flanking region for potential transcriptional activation elements, and examined its expression in nontransformed T-lineage cell populations. The human IL-13 gene was located 12.5-kb upstream of the IL-4 gene and 2-kb downstream of a CpG island. The IL-13 gene 5' flank region included a segment with sequence homology to P elements of the IL-4 promoter involved in transcriptional activation in T cells. Mutation of the IL-13 P element site significantly reduced IL-13 promoter activity in response to T-cell activation. Oligonucleotides containing the IL-13 or IL-4 P element sites specifically bound the transcriptional activator protein, nuclear factor-activated T cells, preformed (NF-ATp), when incubated with nuclear protein extracts from activated T cells. Similar to IL-4, IL-13 mRNA expression was highest in T-cell populations enriched for cells that had previously been primed in vivo or in vitro, indicating that priming increases the expression of the IL-13 and IL-4 genes in a coordinate manner. Because the primed T cells contain higher levels of nuclear NF-ATp, capable of binding to P elements of the IL-4 and IL-13 promoters, than do freshly-isolated T cells, the NF-AT-binding P elements are attractive candidates to mediate the coordinate expression of these two cytokine genes.

摘要

白细胞介素-13(IL-13)和IL-4是由T细胞产生的细胞因子,由人类5号染色体的q23 - 31区域编码。为了研究T细胞对IL-13基因表达的调控,我们分离并测序了人类IL-13基因,分析其5'侧翼区域以寻找潜在的转录激活元件,并检测其在未转化的T系细胞群体中的表达。人类IL-13基因位于IL-4基因上游12.5 kb处,在一个CpG岛下游2 kb处。IL-13基因的5'侧翼区域包含一段与IL-4启动子的P元件具有序列同源性的片段,该元件参与T细胞中的转录激活。IL-13 P元件位点的突变显著降低了T细胞激活后IL-13启动子的活性。当与活化T细胞的核蛋白提取物一起孵育时,含有IL-13或IL-4 P元件位点的寡核苷酸特异性结合转录激活蛋白——预形成的核因子活化T细胞(NF-ATp)。与IL-4相似,IL-13 mRNA表达在富集了先前在体内或体外被致敏细胞的T细胞群体中最高,这表明致敏以协同方式增加了IL-13和IL-4基因的表达。因为与新鲜分离的T细胞相比,致敏的T细胞含有更高水平的能够结合IL-4和IL-13启动子P元件的核NF-ATp,所以NF-AT结合的P元件是介导这两种细胞因子基因协同表达的有吸引力的候选元件。

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