| Soluble expression and characterization of a GFP-fused pea actin isoform(PEAc1) |
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| 作者姓名: | Liu AX Zhang SB Xu XJ Ren DT Liu GQ |
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| 作者单位: | StateKeyLaboratoryofPlantPhysiologyandBiochemistry,CollegeofBiologicalScience,ChinaAgriculturalUniversity,Beijing100094,China |
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| 摘 要: | A pea actin isoform PEAcl with green fluorescent protein (GFP) fusion to its C-terminus and His-tag to its Nterminus, was expressed in prokaryotic cells in soluble form, and highly purified with Ni-Chelating Sepharose^TM Fast Flow column. The purified fusion protein (PEAcl-GFP) efficiently inhibited DNase I activities before polymerization,and activated the myosin Mg-ATPase activities after polymerization. The PEAcl-GFP also polymerized into green fluorescent filamentous structures with a critical concentration of 0.75μM. These filamentous structures were labeled by TRITC-phalloidin, a specific agent for staining actin microfilaments, and identified as having 9 nm diameters by negative staining. These results indicated that PEAc 1 preserved the essential characteristics of actin even with His-tag and GFP fusion, suggesting a promising potential to use GFP fusion protein in obtainning soluble plant actin isoform to analyze its physical and biochemical properties in vitro. The PEAcl-GFP was also expressed in tobacco BY2 cells,which offers a new pathway for further studying its distribution and function in vivo.
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| 关 键 词: | 肌动蛋白 对碘氧基苯甲醚 绿色荧光蛋白 表达 原核细胞?A |
Soluble expression and characterization of a GFP-fused pea actin isoform (PEAc1) |
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| Liu AX,Zhang SB,Xu XJ,Ren DT,Liu GQ.Soluble expression and characterization of a GFP-fused pea actin isoform (PEAc1)[J].Cell Research,2004,14(5):407-414. |
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| Authors: | Liu Ai Xiao Zhang Shao Bin Xu Xiao Jing Ren Dong Tao Liu Guo Qin |
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| Institution: | State Key Laboratory of Plant Physiology and Biochemistry, College of Biological Science, China Agricultural University, Beijing 100094, China. Liu@cau.edu.cn |
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| Abstract: | A pea actin isoform PEAc1 with green fluorescent protein (GFP) fusion to its C-terminus and His-tag to its N-terminus, was expressed in prokaryotic cells in soluble form, and highly purified with Ni-Chelating Sepharose Fast Flow column. The purified fusion protein (PEAc1-GFP) efficiently inhibited DNase I activities before polymerization, and activated the myosin Mg-ATPase activities after polymerization. The PEAc1-GFP also polymerized into green fluorescent filamentous structures with a critical concentration of 0.75 uM. These filamentous structures were labeled by TRITC-phalloidin, a specific agent for staining actin microfilaments, and identified as having 9 nm diameters by negative staining. These results indicated that PEAc1 preserved the essential characteristics of actin even with His-tag and GFP fusion, suggesting a promising potential to use GFP fusion protein in obtaining soluble plant actin isoform to analyze its physical and biochemical properties in vitro. The PEAc1-GFP was also expressed in tobacco BY2 cells, which offers a new pathway for further studying its distribution and function in vivo. |
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| Keywords: | actin isoform polymerization DNase I inhibition myosin Mg-ATPase activation expression |
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