Parameters of heat denaturation and intrinsic fluorescence of barnase and its close homologue, binase in the pH region 2-6 have been determined. The barnase heat denaturation (pH 2.8-5.5) proceeds according to the "all-or-none" principle. Barnase denaturation temperature is lower than that of binase and this difference increases from 2.5 degrees C at pH 5 to 7 degrees C at pH 3. Enthalpy values of barnase and binase denaturation coincide only at pH 4.5-5.5, but as far as pH decreases the barnase denaturation enthalpy decreases significantly and in this respect it differs from binase. The fluorescence and CD techniques do not reveal any distinctions in the local environment of aromatic residues in the two proteins, and the obtained difference in the parameters of intrinsic fluorescence is due to fluorescence quenching of the barnase Trp94 by the His 18 residue, absent in binase. Secondary structures of both native and denaturated proteins also do not differ. Some differences in the barnase and binase electrostatic characteristics, revealed in the character of the dipole moments distribution, have been found.
To elucidate the functional role of some residues in the active site of binase, the extracellular ribonuclease of Bacillus intermedius, we used site-directed mutagenesis. On cleavage of various substrates the catalytic activity of binase mutant His""Glu is 2.0-2.7% of that for native enzyme. The decrease in activity is determined mainly by the decrease in molecular rate constant k,,, with almost unchanged affinity of the enzyme for the substrate, characterized by KM. This is the expected result if His"' acts as an general acid, donating a proton to the leaving group on cleavage of a phosphodiester bond. The replacement of Lysz6 by Ala causes a reduction in the enzyme activity to 13-33%, depending on the substrate. The activity decreases are due to changes in both k,, and KM for poly(1) and poly(A) but in t,, alone for GpA. In the latter case the effect is far less than that seen in the homologous mutation in the closely related enzyme, bamase.
Bacterial ribonucleases from Bacillus amyloliquefaciens and Bacillus intermedius show the specificity towards the nature of a nucleoside at the 03' end of the phoshodiester bond to be split in the preference order G>A+U>C in the cleavage reactions of polynucleotides. It follows from the X-ray data that the substrate guanosine base is bound at the active site of these RNases in the same manner as for high-specificity guanylic RNases. We supposed that the difference in specificity for the two types of RNases is due to the additional hydrogen bond between the protein and a purine base in the case of bacterial guanyl-preferring EWases in contrast to the high-specificity guanylic RNases. To examine this hypothesis we prepared the Ser57+Glu mutant of B. amyloliquefuciens, in which this hydrogen bond is eliminated. Kinetic studies demonstrate that the specificity of this mutant towards guanylic substrates is 35-times greater than that of the wild-type RNases from B. amyloliquefaciens and close to that of RNases TI.
To elucidate the functional role of Arg VP and Arg VT in the enzyme activity of binase, the extracellular ribonuclease of Bacillus intermedius, we used site-directed mutagenesis. On cleavage of various substrates the catalytic activity of binase mutant Arg VT Ala is 2.7U10 Q^7 .7U10 Q times less than that of the native enzyme. The decrease in activity is determined preferentially by the decrease in the molecular rate constant k t with a relatively small change of enzyme-substrate affinity, characterized by K m . This is the expected result if Arg VT acts to lower the energy of a transition state of the reaction. The replacement of Arg VP by Ala causes a 5^19-fold activity decrease, depending on the substrate. We propose that this residue does not have a direct catalytic function in the molecular mechanism of the binase action and that the activity decrease of binase on the replacement of Arg VP by alanine is mediated by the effect of Arg VP on the pK of catalytic residues.z 1998 Federation of European Biochemical Societies.
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