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作 者:莫毅[1,2] 王伟[3] 梁方方 傅冠元[3] 蒋和生[1] Wayne Zhou
机构地区:[1]广西大学动物科学技术学院,广西南宁530004 [2]广西人口和计划生育研究中心,广西南宁530021 [3]美国路易斯安那州立大学生命科学院,美国巴吞鲁日LA70803 [4]广西畜牧研究所,广西南宁530001
出 处:《黑龙江畜牧兽医》2009年第3期17-20,共4页Heilongjiang Animal Science And veterinary Medicine
基 金:美国DERC基金项目
摘 要:为了获得分离纯化shp—1催化活性域蛋白(D1C)并估测其动力学常数,试验选择D1C的转化菌株经IVFG诱导表达、菌体裂解缓冲液悬浮和超声波破碎后,通过HPLC分离纯化D1C蛋白,所得产物进行SDS~PAGE电泳检测,然后以pY作为去磷酸化反应的底物,利用孔雀绿显色法,通过双倒数作图法对纯化的D1C蛋白进行动力学分析。结果表明:试验成功地表达了D1C蛋白,其分子质量约为34.6ku,主要以可溶性蛋白的形式表达;通过HPLC技术可有效地对D1C蛋白进行分离纯化;D1C蛋白的米氏常数Km=2.04mmol/L,催化常数(kcat)=44.98s^-1,特异性常数(kcat/Km)=22.05L/(mmol·s)。To express and purify the catalytic domain of shp - 1 ( name as D1C ) and calculate its kinetic constants. We first expressed DI C from transformed E. coli BL21 bacteria under IPTG induction and purified D1C peptides through HPLC then confirmed by SDS -PAGE. The purified peptides were further subjected to kinetic specificity study using synthetic pY as substratc by malachite green method and analyzed by Lineweaver- Burk plot calculation. From this study, we found D1C peptides were induced to express with soluble state in E coli. BL 21 successfully and purified with HPLC system efficiently. The molecular weigh of D1C was 34.6 ku, and its michaelis constant ( Km ) was 2.04 mmol/L, catalytic constant (kcat) was 44.98 s ^- 1, specific constant (kcat/Km) was 22.05 L/( mmol · s).
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