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A cDNA microarray assessment of gene expression in the liver of rainbow trout (Oncorhynchus mykiss) in response to a handling and confinement stressor

机译:cDNa微阵列评估虹鳟(Oncorhynchus mykiss)肝脏中基因表达对处理和限制应激物的反应

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摘要

A purpose-designed microarray platform (Stressgenes, Phase 1) was utilised to investigate the changes in gene expression within the liver of rainbow trout during exposure to a prolonged period of confinement. Tissue and blood samples were collected from trout at intervals up to 648 h after transfer to a standardised confinement stressor, together with matched samples from undisturbed control fish. Plasma ACTH, cortisol, glucose and lactate were analysed to confirm that the neuroendocrine response to confinement was consistent with previous findings and toudprovide a phenotypic context to assist interpretation of gene expression data. Liver samples for suppression subtractive hybridisation (SSH) library construction were selected from within the experimental groups comprising “early” stress (2–48 h) and “late” stress (96–504 h). In order to reduce redundancy within the four SSH libraries and yield a higher number of unique clones an additional subtraction was carried out. After printing ofudthe arrays a series of 55 hybridisations were executed to cover 6 time points. At 2 h, 6 h, 24 h, 168 h and 504 h 5 individual confined fish and 5 individual control fish were used with control fish only at 0 h. A preliminary list of 314 clones considered differentially regulated over the complete time course was generated by a combination of data analysis approaches and the most significant gene expression changes were found toudoccur during the 24 h to 168 h time period with a general approach to control levels by 504 h. Few changes in expression were apparent over the first 6 h. The list of genes whose expression was significantly altered comprised predominantly genes belonging to the biological process category (response to stimulus) and one cellular component category (extracellular region) and were dominated by so-called acute phase proteins. Analysis of the gene expression profile in liver tissue during confinement revealed a number of significant clusters. The major patterns comprised genes that were up-regulated at 24 h and beyond, the primary examples being haptoglobin, β-fibrinogen and EST10729. Two representative genes from eachudof the six k-means clusters were validated by qPCR. Correlations between microarray and qPCR expression patterns were significant for most of the genes tested. qPCR analysis revealed that haptoglobin expression was up-regulated approximately 8-fold at 24 h and over 13-fold by 168 h.
机译:利用专门设计的微阵列平台(Stressgenes,第1期)来研究虹鳟鱼在长时间禁闭期间肝脏内基因表达的变化。在转移到标准的限制应激源后,在不超过648小时的时间间隔内从鳟鱼中收集组织和血液样本,以及来自不受干扰的对照鱼的匹配样本。分析血浆ACTH,皮质醇,葡萄糖和乳酸,以确认对局限性的神经内分泌反应与先前的发现一致,并提供表型背景来协助解释基因表达数据。从包括“早期”应激(2–48 h)和“晚期”应激(96–504 h)的实验组中选择用于抑制消减杂交(SSH)文库构建的肝样品。为了减少四个SSH库中的冗余并产生更多的唯一克隆,请执行其他减法操作。在打印阵列之后,执行了一系列55次杂交以覆盖6个时间点。在2 h,6 h,24 h,168 h和504 h时,仅在0 h才使用5条单独的密闭鱼和5条单独的对照鱼。通过数据分析方法的组合,得出了在整个时间过程中被差异调节的314个克隆的初步列表,发现在24 h至168 h的时间段内,最重要的基因表达变化是假的,采用一般的控制方法水平504小时。在最初的6小时内,几乎没有表达变化。表达显着改变的基因列表主要包括属于生物过程类别(对刺激的反应)和一个细胞成分类别(细胞外区域)的基因,并且被所谓的急性期蛋白所控制。在封闭期间对肝组织中基因表达谱的分析显示出许多重要的簇。主要模式包括在24小时及以后被上调的基因,主要例子是触珠蛋白,β-纤维蛋白原和EST10729。通过qPCR验证了来自六个k-均值簇的每个 ud的两个代表性基因。芯片和qPCR表达模式之间的相关性对于大多数测试的基因是重要的。 qPCR分析显示触珠蛋白的表达在24小时上调了约8倍,到168小时超过了13倍。

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