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Differential gene expression profiling of mouse skin after sulfur mustard exposure: Extended time response and inhibitor effect.

机译:硫芥子暴露后小鼠皮肤的差异基因表达谱:延长的时间响应和抑制剂作用。

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摘要

Sulfur mustard (HD, SM), is a chemical warfare agent that within hours causes extensive blistering at the dermal-epidermal junction of skin. To better understand the progression of SM-induced blistering, gene expression profiling for mouse skin was performed after a single high dose of SM exposure. Punch biopsies of mouse ears were collected at both early and late time periods following SM exposure (previous studies only considered early time periods). The biopsies were examined for pathological disturbances and the samples further assayed for gene expression profiling using the Affymetrix microarray analysis system. Principal component analysis and hierarchical cluster analysis of the differently expressed genes, performed with ArrayTrack showed clear separation of the various groups. Pathway analysis employing the KEGG library and Ingenuity Pathway Analysis (IPA) indicated that cytokine-cytokine receptor interaction, cell adhesion molecules (CAMs), and hematopoietic cell lineage are common pathways affected at different time points. Gene ontology analysis identified the most significantly altered biological processes as the immune response, inflammatory response, and chemotaxis; these findings are consistent with other reported results for shorter time periods. Selected genes were chosen for RT-PCR verification and showed correlations in the general trends for the microarrays. Interleukin 1 beta was checked for biological analysis to confirm the presence of protein correlated to the corresponding microarray data. The impact of a matrix metalloproteinase inhibitor, MMP-2/MMP-9 inhibitor I, against SM exposure was assessed. These results can help in understanding the molecular mechanism of SM-induced blistering, as well as to test the efficacy of different inhibitors.
机译:芥菜(HD,SM)是一种化学战剂,在数小时内可在皮肤的真皮-表皮交界处引起大量起泡。为了更好地了解SM引起的水疱的进展,在单次高剂量的SM暴露后进行了小鼠皮肤的基因表达谱分析。在SM暴露后的早期和晚期都收集了小鼠耳朵的打孔活检(以前的研究仅考虑了早期)。检查活检组织是否存在病理紊乱,并使用Affymetrix微阵列分析系统进一步分析样品的基因表达谱。使用ArrayTrack对不同表达的基因进行主成分分析和层次聚类分析,结果表明各个组之间的清晰分离。使用KEGG库和Ingenuity Pathway Analysis(IPA)进行的途径分析表明,细胞因子与细胞因子受体的相互作用,细胞粘附分子(CAM)和造血细胞谱系是在不同时间点受到影响的常见途径。基因本体分析确定了最显着改变的生物过程,如免疫反应,炎症反应和趋化性。这些发现与较短时间内的其他报告结果一致。选择了选定的基因用于RT-PCR验证,并显示了微阵列总体趋势中的相关性。检查白介素1 beta的生物学分析,以确认与相应微阵列数据相关的蛋白质的存在。评估了基质金属蛋白酶抑制剂MMP-2 / MMP-9抑制剂I对SM暴露的影响。这些结果可以帮助理解SM引起的水泡的分子机制,以及测试不同抑制剂的功效。

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