作物学报 ›› 2011, Vol. 37 ›› Issue (01): 79-86.doi: 10.3724/SP.J.1006.2011.00079
王明霞1,高翔1,2,*,陈其皎1,2,*,董剑1,2,赵万春1,2,李艳亮1,李敏1
WANG Ming-Xia1,GAO Xiang1,2,*,CHEN Qi-Jiao1,2,*,DONG Jian1,2,ZHAO Wan-Chun1,2,LI Yan-Liang1,LI Min1
摘要: 利用设计合成的特异γ-醇溶蛋白基因引物,采用PCR方法从小麦品种陕253克隆获得一个γ-醇溶蛋白基因(GenBank登录号GQ857626)。序列分析表明,该基因编码产物的II区由于碱基转换产生一个额外的半胱氨酸残基。构建了GQ857626的原核表达载体并转入表达菌株E. coli Rosetta gami B(DE3),IPTG诱导其成功表达。使用HisTrap HP组氨酸标记亲和层析柱纯化该基因的表达产物,并使用4 g粉质仪分析其功能。结果显示,将此纯化蛋白通过氧化还原反应整合到基础面粉后,面团的形成时间缩短,稳定时间减少,弱化度增加,导致主要的粉质指数明显下降,说明该亚基对面团流变学性质整体表现不利。
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