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Differential expression of genes characterizing myofibre phenotype.

机译:表征肌纤维表型的基因的差异表达。

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Skeletal muscle is composed of metabolically heterogeneous myofibres that exhibit high plasticity at both the morphological and transcriptional levels. The objective of this study was to employ microarray analysis to elucidate the differential gene expression between the tonic-'red' anterior latissimus dorsi (ALD) muscle, the phasic-'white' posterior latissimus dorsi (PLD) and 'mixed'-phenotype biceps femoris (BF) in 1-week-and 19-week-old male turkeys. A total of 170 differentially expressed genes were identified in the muscle samples analysed (P<0.05). Gene GO analysis software was utilized to identify top gene networks and metabolic pathways involving differentially expressed genes. Quantitative real-time PCR for selected genes (BAT2D, CLU, EGFR and LEPROT) was utilized to validate the microarray data. The largest differences were observed between ALD and PLD muscles, in which 32 genes were over-expressed and 82 genes were under-expressed in ALD1-PLD1 comparison, and 70 genes were over-expressed and 70 under-expressed in ALD19-PLD19 comparison. The largest number of genes over-expressed in ALD muscles, as compared to other muscles, code for extracellular matrix proteins such as dystroglycan and collagen. The gene analysis revealed that phenotypically 'red' BF muscle has high expression of glycolytic genes usually associated with the 'white' muscle phenotype. Muscle-specific differences were observed in expression levels of genes coding for proteins involved in mRNA processing and translation regulation, proteosomal degradation, apoptosis and insulin resistance. The current findings may have large implications in muscle-type-related disorders and improvement of muscle quality in agricultural species.
机译:骨骼肌由代谢异质性肌纤维组成,在形态学和转录水平上均表现出高可塑性。这项研究的目的是利用微阵列分析来阐明补品-“红色”前背阔肌(ALD)肌肉,相位-“白”后背阔肌(PLD)和“混合”表型二头肌之间的差异基因表达。 1周龄和19周龄的雄性火鸡中的股骨(BF)。在所分析的肌肉样本中共鉴定出170个差异表达基因( P <0.05)。基因GO分析软件用于鉴定涉及差异表达基因的顶级基因网络和代谢途径。利用选定的基因( BAT2D , CLU , EGFR 和 LEPROT )进行实时定量PCR验证芯片数据。在ALD和PLD肌肉之间观察到最大的差异,在ALD1-PLD1比较中32个基因过表达,在82个基因中过表达,在ALD19-PLD19比较中过表达70个基因,在70个表达不足。与其他肌肉相比,在ALD肌肉中过量表达的基因最多,编码的是胞外基质蛋白,例如dystroglycan和胶原蛋白。基因分析显示,表型上的“红色” BF肌肉具有通常与“白色”肌肉表型相关的糖酵解基因的高表达。在编码参与mRNA加工和翻译调节,蛋白质体降解,细胞凋亡和胰岛素抵抗的蛋白质的基因的表达水平中观察到了肌肉特异性差异。目前的发现可能对与肌肉类型相关的疾病和改善农业物种的肌肉质量具有重大意义。

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