Human rhinovirus 2A proteinase mutant and its second-site revertants

The 2A proteinases of human rhinoviruses are cysteine proteinases with marked similarities to serine proteinases. In the absence of a three-dimensional structure, we developed a genetical screening system for proteolytic activity and identified Phe-130 as a key residue. The mutation Phe-130-->Tyr...

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Bibliographic Details
Published in:Biochemical journal 1996-08, Vol.318 ( Pt 1) (1), p.213-218
Main Authors: Luderer-Gmach, M, Liebig, H D, Sommergruber, W, Voss, T, Fessl, F, Skern, T, Kuechler, E
Format: Article
Language:English
Subjects:
Binding Sites
Circular Dichroism
Cysteine Endopeptidases - chemistry
Cysteine Endopeptidases - genetics
Cysteine Endopeptidases - metabolism
Enzyme Stability
Escherichia coli - genetics
Genes, Viral
Genetic Testing
Humans
Kinetics
Lac Operon
Mutagenesis, Site-Directed
Point Mutation
Protein Denaturation
Recombinant Proteins - genetics
Recombinant Proteins - metabolism
rhinovirus
Rhinovirus - enzymology
Temperature
Transformation, Genetic
Viral Proteins
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Summary:The 2A proteinases of human rhinoviruses are cysteine proteinases with marked similarities to serine proteinases. In the absence of a three-dimensional structure, we developed a genetical screening system for proteolytic activity and identified Phe-130 as a key residue. The mutation Phe-130-->Tyr almost completely inhibited enzyme activity at 37 degrees C; activity was, however, partially restored by the following exchanges: Ser-27-->Pro, His-135-->Arg or His-137-->Arg. To investigate this phenotypic reversion, 2A proteinases with the mutations Phe-130-->Tyr, Phe-130-->Tyr/His-135-->Arg, Phe-130-->Tyr/His-137-->Arg, His-135-->Arg or His-137-->Arg were expressed in Escherichia coli and purified. None of these mutations affected the affinity of the enzyme for a peptide substrate. However, the temperature-dependence of enzyme activity, as assayed by cleavage of a peptide substrate and by monitoring the toxicity of the proteinases towards the E. coli strain BL21(DE3), and the structural stability, as monitored by 8-anilino-I-naphthalenesulphonic acid fluorescence and CD spectrometry, were affected. The thermal transition temperatures for both the activity and the stability of the Phe-130-->Tyr 2A proteinase were reduced by about 17 degrees C compared with the wild-type enzyme. The presence of the additional mutations His-135-->Arg or His-137-->Arg in the Phe-130-->Tyr mutant increased temperature stability by 3 degrees C and 6 degrees C respectively. Thus essential interactions exist within the C-terminal domain of human rhinoviral 2A proteinases which contribute to the overall stability and integrity of the enzyme.
ISSN:0264-6021
1470-8728
DOI:10.1042/bj3180213