Sablina E P, Antonov V K
Shemyakin Institute of Bioogranic Chemistry, USSR Academy of Sciences, Moscow.
FEBS Lett. 1991 Jun 3;283(2):291-4. doi: 10.1016/0014-5793(91)80611-6.
Active 3C protease of poliovirus 1(M) was obtained when cloning and expressing fragment HindII-HindIII (bases from 5240 to 6056) of cDNA in vector pTTQ8 in E.coli cells. As shown, fragment 3D of polymerase covalently bound to 3C does not deprive the enzyme of its specific proteolytic activity. The absence of 26 N-terminal amino acids in 3C entails its inactivation. The recombinant 3C protease cleaved peptide bond Gln-Gly not only in virus polyprotein, but also in molecules of beta-galactosidase and bovine catalase.
在大肠杆菌细胞中,将脊髓灰质炎病毒1(M)的活性3C蛋白酶基因的HindII - HindIII片段(cDNA的5240至6056位碱基)克隆并表达于载体pTTQ8时,可获得该蛋白酶。结果表明,与3C共价结合的聚合酶3D片段并不影响该酶的特异性蛋白水解活性。3C蛋白N端缺失26个氨基酸会导致其失活。重组3C蛋白酶不仅能切割病毒多聚蛋白中的Gln - Gly肽键,还能切割β - 半乳糖苷酶和牛过氧化氢酶分子中的该肽键。
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