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Materials and methods (1)E. coli flavohemoglobin gene has been cloned essentially as reported by Membrillo-Hernandez et al.[7] and expressed in E. coli under the control of an IPTG inducible promoter by using a PET11 plasmid.(2)The recombinant protein was purified by means of a three-step chromatographic procedure that avoids ammonium sulfate precipitation and yields >5 mg of pure protein per liter of culture.(3)The E. coli crude extract was loaded onto a DEAE 52 column equilibrated with 10 mM Tris^HCl buffer at pH 8.0 containing 0.1 mM EDTA, 1 mM dithiothreitol and 1 mM potassium cyanide. (4)The flavohemoglobin was eluted with an NaCl gradient at 0.18 M salt concentration. (5)The fractions with flavohemoglobin contents higher than 50%, as judged by SDS^PAGE, were pooled, dialyzed against 5 mM phosphate buffer at pH 7.0 and loaded onto a microceramic hydroxylapatite (Bio-Rad, Hercules, CA, USA) column equilibrated with the same buffer. (6)A 5^50 mM phosphate gradient (pH 7.0) was applied and the protein eluted at a buffer concentration of 15 mM.(7) The fractions containing more than 90% flavohemoglobin were loaded directly onto a DEAE-Toyo Pearl (Toso Haas) column equilibrated in 15 mM phosphate buffer and eluted with an NaCl gradient (0^0.25 M). (8)The protein obtained was s98% pure on SDS^PAGE and was fully saturated with flavin cofactor as judged from the ratio (0.27) between the absorption peak of the heme cyanide complex (419 nm) and the oxidized flavin peak (480 nm). ÕâƪÎÄÏ׵ķ½·¨Óеĵط½¿´²»¶®£¬²»ÖªµÀ¸ÃÔõô±í´ï²Å׼ȷ£¬Çë¸ßÊÖ°ïæ·ÒëÒ»ÏÂ3¡¢5¡¢7¡¢8¾ä»°¡£ ·Ç³£¸Ðл´ó¼ÒµÄ°ïÖúÀ²~~~ ¿ÉÄÜÄÚÈÝÓеã¶à£¬Ï£Íû×ö¹ýµ°°×µÄͬѧÄÜ°ïæ¿´¿´£¬ÔÙ´Îл¹ý |
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