In GMGE cells transfected with pcDNA3.1-GLUT1 and pcDNA3.1-GLUT12 simultaneously, which may be attributed to that GLUT1 was mainly distributed in cell membrane, while GLUT12 was always expressed in endoplasmic reticulum or Golgi apparatus. Enough glucose in endoplasmic reticulum or Golgi apparatus alone was unable to guarantee the activation of protein synthesis. Only when glucose is both abundant in the cytoplasm and Golgi apparatus, theFunctional Analysis of GLUT1 and GLUTtranslation elongation will be promoted to start protein synthesis. Vps34, encoded by PIK3C3, is necessary for mTORC1 activity in response to amino acids sensing in cultured cells [18]. The overexpression of GLUTs could enhance AATs expression to absorb more amino acids, which would then induce the upregulation of PIK3C3. As inhibitor of mTOR signaling [18], the decrease expression of RHEB could in turn stimulate the activation of protein synthesis. Besides mTOR signaling, the JakStat signaling pathway could also take part in glucose and protein metabolism in MGE cells [43]. However, the overexpression of GLUT1 or GLUT12 did not affect STAT5B expression. Moreover, PRLR expression was significantly down-regulated compared to control group. We guess that enhanced AATs expression stimulated the absorption of amino acids, and the GMGE cells used the PRLR pathway as a negative regulation way to balance the intracellular condition. The detailed mechanism should be determined in future.strongly similar properties-scoring .0.5 in the Gonnet PAM 250 matrix. A. (period) indicates conservation between groups of weakly similar properties-scoring = ,0.5 in the Gonnet PAM 250 matrix. (TIF)Figure S3 Prediction of transmembrane helices analysis of goat GLUT1 (A), and bovine GLUT1 (B), goat GLUT12 (C) and bovine GLUT12 (D). Red line means transmembrane region, blue line means inside region and pink line means outside region. Vertical coordinate means probability of transmembrane helices, and horizontal coordinate means AA sequence. (TIF) Figure S4 pGLUT1-GFP (A) and pGLUT12-RFP (B) vector construction diagrams. (TIF) Figure S5 Detection of GLUT1 (A: inherent GLUT1, B: the overexpression of GLUT1, C: the total expression of GLUT1) and GlUT12 in GMGE cells (D: inherent GLUT12, E: the overexpression of GLUT12, F: the total 23148522 expression of GLUT12). pGLUT1-GFP and pGLUT12-RFP were transfected into GMGE cells (GT1-GFP-GMGE cells and GT12-GFP-GMGE cells) respectively to detect the overexpression part of the GLUT1 (B) and GLUT12 (E) under the fluorescence microscope. The overexpression of GLUT1 and GLUT12 were both mainly distributed around the nuclear membrane. (TIF)Supporting InformationFigure S1 The partial cDNA and deduced amino acid sequence of GLUT1 and GLUT12. In the cDNA sequence uppercase letters represent the 5′ and 3′ untranslated regions and lowercase letters represent the coding region. The predicted amino acid sequences shown in uppercase letters are beneath the coding sequences. (A) N-45 was the predicted Terlipressin site N-glycosylation site highlighted in the red AKT inhibitor 2 circle. (B) N-375, 387, 400 and 405 were the predicted Nglycosylation sites highlighted in the red circle. (TIF) Figure S2 Multiple sequence alignment of the deduced aminoAuthor ContributionsConceived and designed the experiments: Q. Yu Q. Yang. Performed the experiments: Q. Yu LZ QT. Analyzed the data: LZ WH. Contributed reagents/materials/analysis tools: Q. Yu JL QZ. Wrote the paper: Q. Yu.acid sequences of goat GLUT1 and GLUT12 wit.In GMGE cells transfected with pcDNA3.1-GLUT1 and pcDNA3.1-GLUT12 simultaneously, which may be attributed to that GLUT1 was mainly distributed in cell membrane, while GLUT12 was always expressed in endoplasmic reticulum or Golgi apparatus. Enough glucose in endoplasmic reticulum or Golgi apparatus alone was unable to guarantee the activation of protein synthesis. Only when glucose is both abundant in the cytoplasm and Golgi apparatus, theFunctional Analysis of GLUT1 and GLUTtranslation elongation will be promoted to start protein synthesis. Vps34, encoded by PIK3C3, is necessary for mTORC1 activity in response to amino acids sensing in cultured cells [18]. The overexpression of GLUTs could enhance AATs expression to absorb more amino acids, which would then induce the upregulation of PIK3C3. As inhibitor of mTOR signaling [18], the decrease expression of RHEB could in turn stimulate the activation of protein synthesis. Besides mTOR signaling, the JakStat signaling pathway could also take part in glucose and protein metabolism in MGE cells [43]. However, the overexpression of GLUT1 or GLUT12 did not affect STAT5B expression. Moreover, PRLR expression was significantly down-regulated compared to control group. We guess that enhanced AATs expression stimulated the absorption of amino acids, and the GMGE cells used the PRLR pathway as a negative regulation way to balance the intracellular condition. The detailed mechanism should be determined in future.strongly similar properties-scoring .0.5 in the Gonnet PAM 250 matrix. A. (period) indicates conservation between groups of weakly similar properties-scoring = ,0.5 in the Gonnet PAM 250 matrix. (TIF)Figure S3 Prediction of transmembrane helices analysis of goat GLUT1 (A), and bovine GLUT1 (B), goat GLUT12 (C) and bovine GLUT12 (D). Red line means transmembrane region, blue line means inside region and pink line means outside region. Vertical coordinate means probability of transmembrane helices, and horizontal coordinate means AA sequence. (TIF) Figure S4 pGLUT1-GFP (A) and pGLUT12-RFP (B) vector construction diagrams. (TIF) Figure S5 Detection of GLUT1 (A: inherent GLUT1, B: the overexpression of GLUT1, C: the total expression of GLUT1) and GlUT12 in GMGE cells (D: inherent GLUT12, E: the overexpression of GLUT12, F: the total 23148522 expression of GLUT12). pGLUT1-GFP and pGLUT12-RFP were transfected into GMGE cells (GT1-GFP-GMGE cells and GT12-GFP-GMGE cells) respectively to detect the overexpression part of the GLUT1 (B) and GLUT12 (E) under the fluorescence microscope. The overexpression of GLUT1 and GLUT12 were both mainly distributed around the nuclear membrane. (TIF)Supporting InformationFigure S1 The partial cDNA and deduced amino acid sequence of GLUT1 and GLUT12. In the cDNA sequence uppercase letters represent the 5′ and 3′ untranslated regions and lowercase letters represent the coding region. The predicted amino acid sequences shown in uppercase letters are beneath the coding sequences. (A) N-45 was the predicted N-glycosylation site highlighted in the red circle. (B) N-375, 387, 400 and 405 were the predicted Nglycosylation sites highlighted in the red circle. (TIF) Figure S2 Multiple sequence alignment of the deduced aminoAuthor ContributionsConceived and designed the experiments: Q. Yu Q. Yang. Performed the experiments: Q. Yu LZ QT. Analyzed the data: LZ WH. Contributed reagents/materials/analysis tools: Q. Yu JL QZ. Wrote the paper: Q. Yu.acid sequences of goat GLUT1 and GLUT12 wit.
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