Subject(s)
Carbonic Anhydrases/metabolism , Plants/enzymology , Acetates/pharmacology , Acetazolamide/analogs & derivatives , Acetazolamide/pharmacology , Affinity Labels , Binding Sites , Bromine , Carbonic Anhydrase Inhibitors , Dithionitrobenzoic Acid/pharmacology , Kinetics , Mercaptoethanol/pharmacology , Pyruvates/pharmacology , Structure-Activity Relationship , Sulfhydryl Compounds/metabolismABSTRACT
Spinach carbonic anhydrase has been purified by modification and extension of a published method (Pocker, Y., and Ng. J. S. U. (1973) Biochemistry 12, 5127-5134), using (NH4)2SO4 precipitation and chromatography on DEAE-cellulose, agarose, and DEAE-Sephadex. The enzyme so obtained was homogeneous by criteria of both standard and sodium dodecyl sulfate polyacrylamide gel electrophoresis and of constant specific activity throughout the elution profile on DEAE-Sephadex chromatography. The enzyme has an apparent Mr of 212,000 by gel filtration on Sephadex G-200, a Mr of 26,000 by sodium dodecyl sulfate electrophoresis, and each of the subunits contains approximately 1 g atom of zinc. These data and the excellent correlation between the number of lysine and arginine residues per subunit, and the number of tryptic peptides obtained by peptide mapping, suggest that spinach carbonic anhydrase is an octamer consisting of identical or very similar subunits. Its amino acid composition is similar to parsley carbonic anhydrase; both contain large numbers of half-cystine residues relative to erythrocyte carbonic anhydrases. The spinach enzyme is devoid of disulfide bonds. The enzyme is stable around neutrality at -14 degrees, as a suspension in saturated (NH4)2SO4 solution.
Subject(s)
Carbonic Anhydrases/isolation & purification , Plants/enzymology , Amino Acids/analysis , Methods , Molecular Weight , Peptide Fragments , Trypsin , Zinc/analysisSubject(s)
Acetazolamide/analogs & derivatives , Carbonic Anhydrases , Affinity Labels , Amino Acids/analysis , Animals , Apoenzymes , Binding Sites , Carbonic Anhydrases/metabolism , Cattle , Cobalt , Hydrogen-Ion Concentration , Kinetics , Peptide Fragments/analysis , Protein Binding , Spectrophotometry , ZincABSTRACT
In order for clinical chemistry to attain full stature as a profession, and clinical biochemistry to become front rank as a discipline, the future education and training of clinical biochemists will require (i) that we achieve recognition and support from our Universities and Hospitals and, where possible, the establishment of Chairs in Clinical Biochemistry, (ii) that we have the resources to attract appropriately qualified physicians and scientists to the staff, (iii) that good courses are developed on the "bio-chemistry of human diseases", "analytical clinical chemistry" and "laboratory administration and management", as a minumum, (iv) that we have the capacity to attract good students for graduate research experience and postgraduate students (both MD and PhD) for professional training and (v) that funds are made available to support these students.
Subject(s)
Chemistry, Clinical/education , Curriculum , Education, GraduateABSTRACT
The reversible complex between the metalloenzyme bovine carbonic anhydrase B and the sulfonamide inhibitor acetazolamide can be "frozen" irreversibly by the addition of a covalent bond between the methyl group of the inhibitor and the tau-nitrogen of histidine-64. In both cases the inhibited enzyme is inactive as an esterase toward p-nitrophenyl propionate at physiological pH but retains activity controlled by an ionization in the protein exhibiting a pK-a greater than 10. Similarly, both the covalently and reversibly inhibited enzymes in which the catalytically essential Zn(II) ion has been replaced with Co(II) display the same visible absorption spectrum which is invariant over the pH range from 5 to 12. The evidence therefore indicates that the position of the acetazolamide moiety in the active site is independent of both pH and the presence of the covalent bond to histidine-64. Moreover, when reversibly bound, this inhibitor has been shown to replace the water molecule (or hydroxide ion) known to occupy the fourth coordination position of the metal ion and frequently implicated in the catalytic mechanism of carbonic anhydrases. Thus, the activity exhibited by the inhibited enzymes and consequently the second rise observed in the pH rate profile of the native enzyme above pH 0 cannot reflect the ionization of such a water molecule in contrast to what has been postulated previously (Pocker, Y., and Storm, D. R. (1968) Biochemistry 7, 1202-1214). Displacement of the zinc-bound solvent molecule rather than the alkylation of histidine-64 is suggested, however, as the cause of the inactivation of the alkylated enzyme round neutrality. Taken together, the biphasic pH rate profile of native bovine carbonic anhydrase B as well as the activity retained by the alkylated enzyme above pH 9 are best described by a model in which two groups in the enzyme ionize independently, thereby raising the possibility that the high pH activity is controlled by an ionization outside the active site region of the enzyme. Above pH 9.5 the pK; for the reversible interaction between native carbonic anhydrase and acetazolamide falls off linearly with increasing pH. The slope of --1.56 suggests that, among other factors, more than one ionization is responsible for the descending limb of the pH-i-pH profile.
Subject(s)
Acetazolamide/pharmacology , Carbonic Anhydrases/metabolism , Animals , Cattle , Cobalt/pharmacology , Hydrogen-Ion Concentration , Kinetics , Nitrophenols/metabolism , Propionates/metabolism , Protein Binding , Spectrophotometry , Zinc/pharmacologyABSTRACT
Partial inactivation of tau-dinitrophenylhistidine-200 human carbonic anhydrase B, induced by visible light, followed first order kinetics (k(app) = 6.05 times 10-2 min-1). After 50 min the tau-dinitrophenylhistidine (tau-DNP-histidine) content decreased to a negligible level, but the illuminated enzyme retained, at pH 7.6, approximately 9.2 percent of the esterase activity of the native enzyme. The following lines of evidence suggest that the loss of activity results from the destruction of tau-DNP-histidine-200. (1) No significant loss of amino acid other than tau-DNP-histidine was detected after illumination. (2) The rate of loss of activity correlated well with the loss of tau-DNP-histidine. (3) In the photooxidized enzyme the DNP moiety was retained but had lost the characteristic sensitivity of tau-DNP-histidine to nucleophilic attack. Titration of the illuminated enzyme with acetazolamide indicated that the residual activity is an intrinsic property of the modified enzyme. The chromatographically purified photooxidized enzyme migrated as a single band on isoelectrofocusing in polyacylamide gel, and at pH 7.6 possessed 7.5 percent esterase activity relative to the native enzyme. By establishing effective destruction of histidine-200, it can be concluded that neither the pi N nor, as previously shown, the tau N of histidine-200 is critical for the catalysis.
Subject(s)
Carbonic Anhydrases , Acetazolamide/pharmacology , Amino Acids/analysis , Carbonic Anhydrases/analysis , Carbonic Anhydrases/metabolism , Esterases/metabolism , Histidine/analogs & derivatives , Humans , Hydrogen-Ion Concentration , Isoelectric Focusing , Light , Mercaptoethanol/pharmacology , Nitrobenzenes , Oxidation-Reduction , Photochemistry , Time FactorsABSTRACT
We have shown that nuclei isolated by two methods contain grossly different amounts of cyclic AMP-dependent histone kinase activity. Repeated washing of the isolated nuclei with a low ionic strength buffer removed the majority of the cyclic AMP-dependent histone kinase and cyclic AMP binding activity. Nuclear cyclic AMP-dependent histone kinase activity accounted for only 0.42% of the total cytoplasmic enzyme activity. Similarly, the lactate dehydrogenase activity associated with liver nuclei represented only 0.07% of the total cytoplasmic activity. The isolated liver nuclei contained only 0.27% of the total homogenate glutamate dehydrogenase activity and 1.7%of the total homogenate glucose-6-phosphatase activity. The cyclic AMP-dependent histone kinase behaves as a cytoplasmic rather than a nuclear enzyme. We have also shown that using crude extracts, one can achieve separation of the two nuclear casein kinases, NI and NII, on sucrose density gradients in the presence of 0.5M NaCl. Nuclear casein kinases NI and NII had sedimentation coefficients of 3.0 and 593 S, respectively, in the presence of 0.5 M NaCl. Under conditions of low ionic strength, all of the casein kinase activity in the crude nuclear extract sedimented as one peak with a seminentation coefficient of 7.3 S. The aggregation-disaggregation which occurred in the crude extract was reversible and was mainly due to the aggregative and disaggregative properties of casein kinase NII. The two nuclear casein kinases have different affinities for chromatin. When nuclei were disrupted in a hypotonic solution and extracted with a buffercontaining 0.14 M NaCl, casein kinase NII could be completely extracted from the viscous nuclear material. Although a significant amount of casein kinase NI was extracted by the buffer containing 0.14 M NaCl, re-extraction of the nuclear material with a buffer containing 0.5 M NaCl yielded substantial amounts of casein kinase NI, and a final extraction with a buffer containing 1.0 M NaCl yielded measurable amounts of casein kinase NI. No casein kinase NII activity could be detected in the 0.5 M and 1.0M NaCl extracts.
Subject(s)
Cell Nucleus/metabolism , Liver/metabolism , Protein Kinases/metabolism , Animals , Caseins , Cell Fractionation , Centrifugation, Density Gradient , Chromatography, Ion Exchange , Cyclic AMP/pharmacology , Enzyme Activation/drug effects , Histones , Protein Kinases/isolation & purification , Rats , Sodium Chloride , Subcellular Fractions/enzymologyABSTRACT
An in vitro assay system has been established to study acetylation and phosphorylation of nuclear proteins from isolated nuclei. Phosphorylation of neclear proteins reached a peak within 5 min while maximum acetylation occurred about 10 min later. The rate of acetylation of liver nuclear proteins in 15 min incubation was significantly higher in "old" mice (29 mo) than in "young" mice (2 mo), while there was no difference in phosphorylation. When nuclear histones were fractionated by polyacrylamide-urea electrophoresis the acetylation of histone F3 was increased in "old" mice to 129% and F2al to 112% of the values in "young" mice. Acetylation of phenol-soluble nuclear acidic proteins was increased to 250% and phosphorylation to 138% in "old" mice as compared to "young" mice. This increase in covalent modification of acidic proteins was found in tow specific fractions when separated by SDS-polyacrylamide gel electrophoresis. By contrast, the labeling of nucleoplasmic proteins, soluble in 0.14 M NaCl, showed no significant difference between the two ages.