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机构地区:[1]上海海洋大学食品学院/上海水产品加工及贮藏工程技术研究中心,上海201306
出 处:《福建农林大学学报(自然科学版)》2017年第1期81-88,共8页Journal of Fujian Agriculture and Forestry University:Natural Science Edition
基 金:上海市教育委员会产学研项目(15CXY30);农业部都市农业(南方)重点实验室开放项目(UA201307);上海市交叉学科研究生拔尖创新人才培养平台项目(B5201120040);上海市2015高校内涵建设项目(A2018150009)
摘 要:从鲤鱼鳃组织中分离克隆到一种新的g型溶菌酶同工型基因(CLYG).该基因的全长cDNA为558 bp,除去终止密码子,编码185个氨基酸,推断的氨基酸序列没有信号肽,含3个催化位点(谷氨酸73、脯氨酸86和天冬氨酸97),具有鱼类g型溶菌酶的基本特征.通过PCR方法在CLYG基因的5'和3'端分别引入XhoⅠ和XbaⅠ酶切位点.扩增到的目的片段与表达载体pPICZαA连接构建重组表达载体pPICZαA-CLYG后,电转至毕赤酵母X-33,筛选得到的阳性转化子在1.0%甲醇、29℃、pH 6.0的条件下诱导表达72 h,获得重组体CLYG.SDS-PAGE和蛋白质印迹分析显示,在毕赤酵母中成功表达了重组体CLYG.G-type lysozyme plays an important role in fishes immune response against microbial invasion. In the present study, a new g-type lysozyme isofor^n gene ( CLYG) w as separated from common carp ( Cyprinus ca rp io ) gill. T h e full-length c D N A of CLYG is 558 bp, which encodes 185 amino acid residues. The amino acid sequence deduced from the cDNA of CLYG contains 3 catalytic res-idues (Glu73, Pro86 and Asp97) without any signal peptide, which is similar to those of other teleost species. Subsequently, Xho I and Xba I restriction sites were added to the 5r and 3r ends of CLYG gene by P C R , respectively. After that, the expected fragment was ligated with expression vector pPICZaA, and followed by being transfor^med into competent P ich ia pastoris X - 3 3 cells. Then recombinant CLYG was induced in 1.0% methanol under pH 6.0 at 29 ^ for 72 h. SDS-PAGE analysis and Western blot anal-ysis demonstrated that the recombinant CLYG was successfully expressed.
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