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首页> 外文期刊>International immunopharmacology >Analysis of gene expression induced by irritant and sensitizing chemicals using oligonucleotide arrays.
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Analysis of gene expression induced by irritant and sensitizing chemicals using oligonucleotide arrays.

机译:使用寡核苷酸阵列分析由刺激性和致敏化学物质诱导的基因表达。

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Chemical-induced allergy continues to be an important occupational health problem. Despite decades of investigation, the molecular mechanisms underlying chemical-induced hypersensitivity and irritancy remain unclear because of the complex interplay between properties of different chemicals and the immune system. In this study, gene expression induced by toluene diisocyanate (TDI, a primarily IgE-inducing sensitizer), oxazolone (OXA, a cell-mediated hypersensitivity inducing sensitizer), or nonanoic acid (NA, a non-sensitizing irritant) was investigated using gene arrays. Female BALB/c mice were dermally exposed on the ears once daily for 4 consecutive days. On day 5, the lymph nodes draining the exposure sites were collected and used for RNA extraction and subsequent hybridization to Affymetrix Mu6500 oligonucleotide arrays. Of the 6519 genes on the arrays, there were 44, 13, and 51 genes in the TDI-, OXA-, and NA-exposed samples, respectively, that displayed a minimum of twofold change in expression level relative to the vehicle control. There were 32, 19, and 19 genes that were differentially expressed (with a minimum of twofold change) between TDI and OXA, TDI and NA, OXA and NA, respectively. The differentially expressed genes include immune response-related genes, transcriptional factors, signal transducing molecules, and Expressed Sequence Tags. Based on the gene array results, candidate genes were further evaluated using RT-PCR. There was only about 47% concordance between the gene array and RT-PCR results.
机译:化学诱导的过敏仍然是重要的职业健康问题。尽管进行了数十年的研究,但由于不同化学物质的特性与免疫系统之间复杂的相互作用,导致化学性超敏反应和刺激性的分子机制仍然不清楚。在这项研究中,使用基因研究了由甲苯二异氰酸酯(TDI,主要是诱导IgE的敏化剂),恶唑酮(OXA,一种细胞介导的超敏性诱导敏化剂)或壬酸(NA,一种非敏化刺激剂)诱导的基因表达。数组。每天一次将雌性BALB / c小鼠的耳朵在皮肤上暴露一次,连续4天。在第5天,收集引流暴露部位的淋巴结,用于RNA提取和随后与Affymetrix Mu6500寡核苷酸阵列的杂交。在阵列上的6519个基因中,在TDI,OXA和NA暴露的样品中分别有44、13和51个基因,相对于赋形剂对照,它们的表达水平变化最小。在TDI和OXA,TDI和NA,OXA和NA之间分别有32个,19个和19个基因差异表达(最少有两倍变化)。差异表达的基因包括与免疫反应相关的基因,转录因子,信号转导分子和表达序列标签。根据基因阵列结果,使用RT-PCR进一步评估候选基因。基因阵列和RT-PCR结果之间只有大约47%的一致性。

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