Liebig H D, Skern T, Luderer M, Sommergruber W, Blaas D, Kuechler E
Institute of Biochemistry, University of Vienna, Austria.
Proc Natl Acad Sci U S A. 1991 Jul 15;88(14):5979-83. doi: 10.1073/pnas.88.14.5979.
Many virally encoded proteinases cleave themselves out of a polyprotein, with cleavage occurring usually at their own N terminus. This property was used to develop an in vivo screening system using the lacZ gene fragment of M13mp18. When a fusion protein of the alpha fragment of beta-galactosidase and an active 2A proteinase of human rhinovirus 2 was expressed, alpha complementation was not affected, as the 2A proteinase cleaved itself off the alpha fragment. However, fusion of an inactive 2A prevented alpha complementation, as the 2A polypeptide remained fused to the alpha fragment. After random mutation of the 2A gene by PCR amplification, mutants were screened; M13 phage defective in alpha complementation were obtained at an efficiency of 5% and were shown to contain mutated 2A genes. Intermolecular cleavage was then examined by expressing an alpha fragment-inactive proteinase fusion protein as substrate for an active 2A proteinase expressed from an M13 vector. alpha complementation indicated intermolecular processing of the 2A cleavage site on the alpha fragment-inactive proteinase fusion protein. This versatile system thus allows the high-density screening of both active and inactive proteinase mutants, cleaving either intramolecularly or intermolecularly, and should be applicable to other proteinases of high specificity.
许多病毒编码的蛋白酶会将自身从多聚蛋白中切割出来,切割通常发生在它们自己的N端。利用这一特性,人们开发了一种使用M13mp18的lacZ基因片段的体内筛选系统。当表达β-半乳糖苷酶α片段与人鼻病毒2的活性2A蛋白酶的融合蛋白时,α互补不受影响,因为2A蛋白酶会将自身从α片段上切割下来。然而,无活性2A的融合会阻止α互补,因为2A多肽仍与α片段融合。通过PCR扩增对2A基因进行随机突变后,筛选突变体;获得了α互补缺陷的M13噬菌体,并显示其含有突变的2A基因。然后,通过表达α片段-无活性蛋白酶融合蛋白作为M13载体表达的活性2A蛋白酶的底物,来检测分子间切割。α互补表明α片段-无活性蛋白酶融合蛋白上2A切割位点的分子间加工。因此,这个通用系统允许对活性和无活性蛋白酶突变体进行高密度筛选,这些突变体可以进行分子内或分子间切割,并且应该适用于其他高特异性的蛋白酶。
