Transcriptome analyses of liver in newly-hatched chicks during the metabolic perturbation of fasting and re-feeding reveals THRSPA as the key lipogenic transcription factor

被引:21
作者
Cogburn, Larry A. [1 ]
Trakooljul, Nares [1 ,2 ]
Wang, Xiaofei [3 ]
Ellestad, Laura E. [4 ,5 ]
Porter, Tom E. [5 ]
机构
[1] Univ Delaware, Dept Anim & Food Sci, Newark, DE 19717 USA
[2] Leibniz Inst Farm Anim Biol, Inst Genome Biol, Wilhelm Stahl Allee 2, D-18196 Dummerstorf, DE, Germany
[3] Tennessee State Univ, Dept Biol Sci, Nashville, TN 37209 USA
[4] Univ Georgia, Dept Poultry Sci, Athens, GA 30602 USA
[5] Univ Maryland, Dept Avian & Anim Sci, College Pk, MD 20742 USA
基金
美国农业部;
关键词
Up-stream regulators; Target genes; Lipid metabolism; Lipolysis; Lipogenesis; Thermogenesis; Gene interaction networks; Homeorhesis; Spot 14 (THRSPA); THRSP paralogs; Metabolic switch; ying-yang metabolic regulation; Reciprocal inhibition; activation; FATTY-ACID SUPPRESSION; S14; GENE-TRANSCRIPTION; FUNCTIONAL GENOMICS; MICROARRAY DATA; X RECEPTOR; EXPRESSION; DISCOVERY; CHEMERIN; GLUCOSE; THERMOGENESIS;
D O I
10.1186/s12864-020-6525-0
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Background The fasting-refeeding perturbation has been used extensively to reveal specific genes and metabolic pathways that control energy metabolism in the chicken. Most global transcriptional scans of the fasting-refeeding response in liver have focused on juvenile chickens that were 1, 2 or 4 weeks old. The present study was aimed at the immediate post-hatch period, in which newly-hatched chicks were subjected to fasting for 4, 24 or 48 h, then refed for 4, 24 or 48 h, and compared with a fully-fed control group at each age (D1-D4). Results Visual analysis of hepatic gene expression profiles using hierarchical and K-means clustering showed two distinct patterns, genes with higher expression during fasting and depressed expression upon refeeding and those with an opposing pattern of expression, which exhibit very low expression during fasting and more abundant expression with refeeding. Differentially-expressed genes (DEGs), identified from five prominent pair-wise contrasts of fed, fasted and refed conditions, were subjected to Ingenuity Pathway Analysis. This enabled mapping of analysis-ready (AR)-DEGs to canonical and metabolic pathways controlled by distinct gene interaction networks. The largest number of hepatic DEGs was identified by two contrasts: D2FED48h/D2FAST48h (968 genes) and D2FAST48h/D3REFED24h (1198 genes). The major genes acutely depressed by fasting and elevated upon refeeding included ANGTPL, ATPCL, DIO2, FASN, ME1, SCD, PPARG, SREBP2 and THRSPA-a primary lipogenic transcription factor. In contrast, major lipolytic genes were up-regulated by fasting or down-regulated after refeeding, including ALDOB, IL-15, LDHB, LPIN2, NFE2L2, NR3C1, NR0B1, PANK1, PPARA, SERTAD2 and UPP2. Conclusions Transcriptional profiling of liver during fasting/re-feeding of newly-hatched chicks revealed several highly-expressed upstream regulators, which enable the metabolic switch from fasted (lipolytic/gluconeogenic) to fed or refed (lipogenic/thermogenic) states. This rapid homeorhetic shift of whole-body metabolism from a catabolic-fasting state to an anabolic-fed state appears precisely orchestrated by a small number of ligand-activated transcription factors that provide either a fasting-lipolytic state (PPARA, NR3C1, NFE2L2, SERTAD2, FOX01, NR0B1, RXR) or a fully-fed and refed lipogenic/thermogenic state (THRSPA, SREBF2, PPARG, PPARD, JUN, ATF3, CTNNB1). THRSPA has emerged as the key transcriptional regulator that drives lipogenesis and thermogenesis in hatchling chicks, as shown here in fed and re-fed states.
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