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首页> 外文期刊>BioMed research international >Cloning and Characterization of Spliced Variants of the Porcine G Protein Coupled Receptor 120
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Cloning and Characterization of Spliced Variants of the Porcine G Protein Coupled Receptor 120

机译:猪G蛋白偶联受体120的剪接变异体的克隆与鉴定

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摘要

The polyunsaturated fatty acids (PUFAs) receptor GPR120 exerts a significant impact on systemic nutrient homeostasis in human and rodents. However, the porcine GPR120 (pGPR120) has not been well characterized. In the current study, we found thatpGPR120had 3 spliced variants. Transcript 1 encoded 362-amino acids (aa) wild type pGPR120-WT, which shared 88% homology with human short form GPR120. Transcript 1 was the mainly expressed transcript ofpGPR120. It was expressed predominantly in ileum, jejunum, duodenum, spleen, and adipose. Transcript 3 (coding 320-aa isoform) was detected in spleen, while the transcript 2 (coding 310-aa isoform) was only slightly expressed in spleen. A selective agonist for human GPR120 (TUG-891) and PUFAs activated SRE-luc and NFAT-luc reporter in HEK293T cells transfected with construct for pGPR120-WT but not pGPR120-V2. However, 320-aa isoform was not a dominant negative isoform. The extracellular signal-regulated kinase 1/2 (ERK1/2) phosphorylation levels in cells transfected with construct for pGPR120-WT were well activated by PUFAs, especially n-3 PUFA. These results showed that although pGPR120 had 3 transcripts, transcript 1 which encoded pGPR120-WT was the mainly expressed transcript. TUG-891 and PUFAs, especially n-3 PUFA, well activated pGPR120-WT. The current study contributed to dissecting the molecular regulation mechanisms of n-3 PUFA in pigs.
机译:多不饱和脂肪酸(PUFAs)受体GPR120对人类和啮齿动物的全身营养稳态具有重要影响。但是,猪GPR120(pGPR120)尚未得到很好的鉴定。在当前研究中,我们发现pGPR120具有3个剪接变体。转录本1编码362个氨基酸(aa)野生型pGPR120-WT,与人短型GPR120具有88%的同源性。转录物1是pGPR120的主要表达转录物。它主要在回肠,空肠,十二指肠,脾脏和脂肪中表达。在脾脏中检测到转录本3(编码320-aa亚型),而在脾脏中仅检测到转录本2(编码310-aa亚型)。在用pGPR120-WT而非pGPR120-V2构建体转染的HEK293T细胞中,人GPR120(TUG-891)和PUFA的选择性激动剂激活了SRE-luc和NFAT-luc报道基因。但是,320-aa亚型不是主要的阴性亚型。 PUFA,尤其是n-3 PUFA很好地激活了用pGPR120-WT构建体转染的细胞中的细胞外信号调节激酶1/2(ERK1 / 2)磷酸化水平。这些结果表明,尽管pGPR120具有3个转录物,但是编码pGPR120-WT的转录物1是主要表达的转录物。 TUG-891和PUFA(尤其是n-3 PUFA)活化良好的pGPR120-WT。目前的研究有助于剖析猪中n-3 PUFA的分子调控机制。

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