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Purification of green fluorescent protein using a two-intein system |
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| Authors: | Zhonglin Zhao Wei Lu Baoqing Dun Dan Jin Shuzhen Ping Wei Zhang Ming Chen Ming-Qun Xu Min Lin |
| Institution: | (1) College of Biological Sciences, China Agricultural University, Beijing, 100094, China;(2) Biotechnology Research Institute, Chinese Academy of Agricultural Sciences, Beijing, 100081, China;(3) Institute of Crop Science, Chinese Academy of Agricultural Sciences, Beijing, 100081, China;(4) Biotechnology Research Center, Southwest University, Chongqing, 400716, China;(5) New England Biolabs, Beverly, MA 01915, USA |
| Abstract: | A two-intein purification system was developed for the affinity purification of GFPmut3*, a mutant of green fluorescent protein. The GFPmut3* was sandwiched between two self-cleaving inteins. This approach avoided the loss of the target protein which may result from in vivo cleavage of a single intein tag. The presence of N- and C-terminal chitin-binding domains allowed the affinity purification by a single-affinity chitin column. After the fusion protein was expressed and immobilized on the affinity column, self-cleavage of the inteins was sequentially induced to release the GFPmut3*. The yield was 2.41 mg from 1 l of bacterial culture. Assays revealed that the purity was up to 98% of the total protein. The fluorescence and circular dichroism spectrum of GFPmut3* demonstrated that the purified protein retains the correctly folded structure and function. |
| Keywords: | Intein Protein splicing Green fluorescent protein Protein purification |
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