Literature DB >> 21805523

GFP-based evaluation system of recombinant expression through the secretory pathway in insect cells and its application to the extracellular domains of class C GPCRs.

Yuji Ashikawa1, Makoto Ihara, Noriko Matsuura, Yuko Fukunaga, Yuko Kusakabe, Atsuko Yamashita.   

Abstract

Applications of the GFP-fusion technique have greatly facilitated evaluations of the amounts and qualities of sample proteins used for structural analyses. In this study, we applied the GFP-based sample evaluation to secreted protein expression by insect cells. We verified that a GFP variant, GFPuv, retains proper folding and monodispersity within all expression spaces in Sf9 cells, such as the cytosol, organelles, and even the extracellular space after secretion, and thus can serve as a proper folding reporter for recombinant proteins. We then applied the GFPuv-based system to the extracellular domains of class C G-protein coupled receptors (GPCRs) and examined their localization, folding, and oligomerization upon insect cell expression. The extracellular domain of metabotropic glutamate receptor 1 (mGluR1) exhibited good secreted expression by Sf9 cells, and the secreted proteins formed dimer with a monodisperse hydrodynamic state favorable for crystallization, consistent with the results from previous successful structural analyses. In contrast, the extracellular domains of sweet/umami taste receptors (T1R) almost completely remained in the cell. Notably, the T1R and mGluR1 subfractions that remained in the cellular space showed polydisperse hydrodynamic states with large aggregated fractions, without forming dimers. These results indicated that the proper folding and oligomerization of the extracellular domains of the class C GPCR are achieved through the secretory pathway.
Copyright © 2011 The Protein Society.

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Year:  2011        PMID: 21805523      PMCID: PMC3218366          DOI: 10.1002/pro.707

Source DB:  PubMed          Journal:  Protein Sci        ISSN: 0961-8368            Impact factor:   6.725


  57 in total

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2.  Structural views of the ligand-binding cores of a metabotropic glutamate receptor complexed with an antagonist and both glutamate and Gd3+.

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Review 3.  Quality control and protein folding in the secretory pathway.

Authors:  E Sergio Trombetta; Armando J Parodi
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5.  Crystal structure and association behaviour of the GluR2 amino-terminal domain.

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6.  Structure of the zinc-bound amino-terminal domain of the NMDA receptor NR2B subunit.

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8.  High-resolution Native-PAGE for membrane proteins capable of fluorescence detection and hydrodynamic state evaluation.

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  10 in total

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2.  Highly efficient production of rabies virus glycoprotein G ectodomain in Sf9 insect cells.

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3.  A large-scale expression strategy for multimeric extracellular protein complexes using Drosophila S2 cells and its application to the recombinant expression of heterodimeric ligand-binding domains of taste receptor.

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4.  Taste substance binding elicits conformational change of taste receptor T1r heterodimer extracellular domains.

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5.  Structural basis for perception of diverse chemical substances by T1r taste receptors.

Authors:  Nipawan Nuemket; Norihisa Yasui; Yuko Kusakabe; Yukiyo Nomura; Nanako Atsumi; Shuji Akiyama; Eriko Nango; Yukinari Kato; Mika K Kaneko; Junichi Takagi; Maiko Hosotani; Atsuko Yamashita
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6.  Expression and purification of a functional heteromeric GABAA receptor for structural studies.

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7.  Specific modification at the C-terminal lysine residue of the green fluorescent protein variant, GFPuv, expressed in Escherichia coli.

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9.  An efficient Escherichia coli expression system for the production of a functional N-terminal domain of the T1R3 taste receptor.

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10.  Differential scanning fluorimetric analysis of the amino-acid binding to taste receptor using a model receptor protein, the ligand-binding domain of fish T1r2a/T1r3.

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  10 in total

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