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Protein Characterization of Na+-Independent System L Amino Acid Transporter 3 in Mice

机译:Na +独立系统L氨基酸转运蛋白3在小鼠中的蛋白质表征

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We recently cloned the human Na+-independent system L neutral amino acid transporter LAT3. The aim of the present study was to characterize the molecular nature of mouse LAT3 at the protein level. Isolated mouse LAT3 showed 83% identity to human LAT3. Xenopus oocytes injected with mouse LAT3 cRNA showed the same functional property as human LAT3. Reverse transcriptase-polymerase chain reaction revealed apparent transcripts of mouse LAT3 in the liver, skeletal muscle, and pancreas, an expression pattern identical to that found in humans. Antibody generated against mouse LAT3 detected both 58-kd and 48-kd bands in the sample from liver and only a 48-kd band in skeletal muscle and pancreas. Immunohistochemical study showed its clear localization in the plasma membrane of liver and skeletal muscle, whereas it was only detectable in the endoplasmic reticulum and in crystalline inclusions in pancreatic acinar cells. Starvation induced up-regulation of mouse LAT3 protein and mRNA in both liver and skeletal muscle but not in pancreas. These results suggest that LAT3 may indeed function as an amino acid transporter, transporting branched-chain amino acids from liver and skeletal muscle to the bloodstream and thereby participating in the regulatory system of interorgan amino acid nutrition.
机译:我们最近克隆了人类Na +独立系统L中性氨基酸转运LAT3。本研究的目的是在蛋白质水平上表征小鼠LAT3的分子性质。分离的小鼠LAT3显示出与人LAT3的83%同一性。注射了小鼠LAT3 cRNA的非洲爪蟾卵母细胞显示出与人LAT3相同的功能特性。逆转录酶-聚合酶链反应显示小鼠LAT3在肝脏,骨骼肌和胰腺中有明显的转录本,其表达模式与人类相同。针对小鼠LAT3产生的抗体在肝脏样品中检测到58 kd和48 kd谱带,在骨骼肌和胰腺中仅检测到48 kd谱带。免疫组织化学研究显示其在肝脏和骨骼肌的质膜中清晰定位,而仅在内质网和胰腺腺泡细胞中的结晶包裹物中可检测到。饥饿诱导小鼠肝脏和骨骼肌中胰腺LAT3蛋白和mRNA的表达上调,但胰腺细胞中没有。这些结果表明,LAT3确实可以充当氨基酸转运蛋白,将支链氨基酸从肝脏和骨骼肌转运到血液,从而参与器官间氨基酸营养的调节系统。

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