METABOLISM AND ENZYMOLOGY OF NUCLEIC ACIDS Gene Incl~ding Manipulations METABOLISM AND ENZYMOLOGY OF NUCLEIC ACIDS Including Gene Manipulations Edited by Jan Zelinka and Jozef Balan Slovak Academy of Sciences Bratislava, Czechoslovakia PLENUM PRESS • NEW YORK AND LONDON Library of Congress Cataloging in Publication Data International Symposium on Metabolism and Enzymology of Nucleic Acids In cluding Gene Manipulations (6th: 1987: Smolenice. Czechoslovakia) Metabolism and enzymology of nucleic acids. including gene manipulations edited by Jan Zelinka and Jozef Balan. p. cm. "Proceedings of the Sixth International Symposium on Metabolism and En zymology of Nucleic Acids Including Gene Manipulations. held June 7-11.1987. at Smolenice Castle. Czechoslovakia" - T.p. verso. Sponsored by the Slovak Academy of Sciences. Includes bibliographical references and indexes. ISBN-13: 978-1-4612-8063-7 e-ISBN: 978-1-4613-0749-5 DOl: 10.1007/978-1-4613-0749-5 1. Nucleic acids-Congresses. 2. Nucleases-Congresses. 3. Methylation Congresses. 4. Molecular cloning-Congresses. 5. Gene expression-Congress es. I. Zelinka. J. (Jan) II. Balan. J. (Jozef) III. Siovenska akademia vied. IV. Title. QP620.156 1987 88-39215 574.87'3282-dc19 CIP Proceedings of the Sixth International Symposium on Metabolism and Enzymology of Nucleic Acids. Including Gene Manipulations. held June 7-11. 1987. at Smolenice Castle. Czechoslovakia. This symposium was held under the auspices of the President of the Slovak Academy of Sciences. Academician Vladimir Hajko. © 1988 Plenum Press. New York Softcover reprint of the hardcover 1s t edition 1988 A Division of Plenum Publishing Corporation 233 Spring Street. New York. N.Y. 10013 All rights reserved No part of this book may be reproduced. stored in a retrieval system. or transmitted in any form or by any means. electronic. mechanical. photocopying. microfilming. recording. or otherwise. without written permission from the Publisher OPENING OF THE SYMPOSIUM I would like to open the Sixth International Symposium on Metabolism and Enzymology of Nucleic Acids Including Gene Manipulations, organized by the Institute of Molecular Biology of the Slovak Academy of Sciences under the auspices of Academician Vladimir Hajko, President of the Slovak Academy of Sciences. This symposium, in a similar way as our previous meetings, is part of the multilateral cooperation of the Academies of Sciences of the socialist countries in the field of molecular biology and biochemistry. We are glad to be able to welcome here, at Smo1enice Castle, numerous outstanding scientists from many countries and our friends whom we tradi tionally meet here. Fourteen years have passed since our first symposium in 1973, and tremendous advances have been achieved in the field of the metabolism and enzymology of nucleic acids which have resulted in gene manipulations and have stimulated the formation of modern biotechnologies. We are happy that our Institute has contributed to this development in a modest way. Our work was helped and supported by the organization of these symposia, giving our younger co-workers the opportunity to find new stimulation for the~r work and to get acquaint~d with scientists from other countries, thus fost ering creative international cooperation. It is especially valuable that this cooperation takes place between countries without regard to their socio-economic setup. The scientists who meet here hold different political opinions, but in spite of this, we are long-time friends, we respect and support each other, and each of us contributes to the development of science which serves all of mankind. This is our contribution to world peace and mutual understanding. Let me use this opportunity to thank all our foreign friends who have contributed in the past or are at present contributing to our mutual sci entific successes or are helping us to master new methodological approaches. I would like to wish you a successful meeting and to express my sincere hope that you will feel at home at Smo1enice Castle. J. Zelinka Corresponding Member of the Czechoslovak and Slovak Academy of Sciences Director, Institute of Molecular Biology, Slovak Academy of Sciences v CONTENTS DNA Methylation and DNA Methyltransferase in Wheat H. Follmann. R. Schleicher and J. Balzer 1 The X-Ray Analysis of Ribonuclease Sa J. Seveik. E.J. Dodson. G.G. Dodson and J. Zelinka 9 The Nature of Distribution of Ribonucleotide Reductases H. Follmann. J. Harder and H.P.C. Hogenkamp 19 Cloning. Expression and Nucleotide Sequence of a Gene Encoding a Second Thioredoxin from Corynebacterium nephridii C.J. Lim. J.A. Fuchs, S.C. McFarlan and H.P.C. Hogenkamp 27 Thioredoxin from Streptomyces aureofaciens M. Kollarova, E. Ka~ova, K. Szuttorova, H. Follmann and J. Zelinka 37 Two-Dimensional IH-NMR ~nvestigation of Ribonuclease Tl and the Complexes of RNase Tl with 2'- and 3'- Guanosine Monophosphate H. RUterjans, E. Hoffman, J. Schmidt and J. Simon 43 Nucleoside Phosphotransferase and Nuclease SI' two Enzymes with Acylphosphate Intermediates, but Different Mechanisms H. Witzel, A. Billich, W. Berg. O. Creutzenberg and A. Karreh 55 Probing the Mechanism of Enzyme Action through Specific Amino Acid Substitutions A.J. Wilkinson 63 Site-Specific Restriction Endonuclease Sau BMK I from Streptomyces aureofaciens J. Timko, J. Turna and J. Zelinka 65 The Effects of N4- and C5-Methylation of Cytosine on DNA Physical Properties and Restriction Endonuclease Action V. Butkus, S. Klimasauskas. L. Petrauskiene. Z. Maneliene, L.E. Minchenkova. A.K. Schyolkina and A. Janulaitis 73 Regulation of RNA Synthesis in Yeast: The Stringent Control of Ribosomal RNA Synthesis L.W. Waltschewa and P.V. Venkov 79 In Vitro Study on Ribosome Degradation in Rat Liver E.N. Nikolov and T.K. Nikolov 85 Specific Labelling in the Functional Domain of Elongation Factor EF-Tu from Bacillus stearothermophilus and from Bacillus subtilis J. Jon§k. K. Karas and I. Rychlik 95 GTP Expense at Codon-Specific Translation and During Misreading L.P. Gavrilova and D.G. Kakhniashvili 101 Site-Directed Mutagenesis of Elongation Factor Tu A. Parmeggiani. E. Jacquet. M. Jensen. P.H. Anborgh. R.H. Cool. J. Jon§k and G.W.M. Swart 109 A Site-Mutated rrsD Gene Expression Construct: Impairment of Ribosomal Function J. Sedla~ek. J. Smrt. J. Lakota. I. Rychlik. M. F§bry and O. Melzochova 117 Expression of Prochymosin cDNA in E. coli M. Fabry, P. Ka!par. S. Zadra!il. F. Kapralek and J. Sedla~ek 123 Control of the Cell Cycle Start by Protein Kinase Genes in Saccharomyces cerevisiae H. KUntzel. J. Lisziewicz. A. Godany. E. Hostinov§. H.H. FHrster. M. Trauzold and H. Sternbach 127 Molecular Analysis of Mitochondrial DNA and Cloning of its rDNA Fragments from Tomato Cell Suspension Culture B. Hause. F. Baldauf. K. Stock. C. Wasternack and M. Metzlaff 131 Nucleotide Compartmentation During Synthesis of Cytoplasmic rRNA and tRNA a~ well as Cytoplasmic rRNA and Mitochondrial rRNA in Tomato Cell Suspension Culture B. Hause and C. Wasternack 137 Intracellular Location of some Purine- and Pyrimidine Metabolizing Enzymes in Plant Cells C. Wasternack. R. Walther. K. Glund. A. Guranowski. H. Tintemann and J. Miersch 143 Some Properties of Dinucleoside Oligophosphate Phosphorylase from Euglena gracilis A. Guranowski. E. Starzynska and C. Wasternack 149 Expression of Genes Coding for Novobiocin Biosynthesis and Novobiocin Resistance in Streptomyces niveus D.A. Ritchie. K.E. Cushing. P.G. Logan and J.I. Mitchell 155 Chromosomal Rearrangements Affecting the Regulation of Uridine Phosphorylase Gene Expression in Escherichia coli A.S. Mironov. S.T. Kulakauskas. V.V. Sukhodolets 161 Repeated Sequences in Chromosomal DNA of Streptomyces aureofaciens 2201 A. Godany. P. Prista!. J. Muchova and J. Zelinka 167 viii Stable Gene Duplication by "Puzzle" Shot Gun Cloning in Inverted Repeats of a Streptococcal Plasmid G.S. Steinborn 173 Different Types of Repetitive Elements in Mammalian Genome: Cloning and Characterization of cDNA Copies of Transcripts Containing Repetitive Sequences A.P. Ryskov, P.L. Ivanov, O.N. Tokarskaya, A.V. Akulichev, E.T. Jumanova, A.G. Jincharadze and L.V. Verbovaya 175 Nucleotide Sequence Analysis of the 5'-End of Chicken c-myb Gene P. Urbanek, M. Dvofak, M. Travni~ek, P. Bartfin~k and V. Pa~es 183 Cloning and Characterization of Human Genes Expressed in Neural Cells S.A. Limborska, P.A. Slominsky, N.E. Maleeva and S.A. Korneev 191 Detection of a ~-Globin Intron Mutation in a ~-Thalassemic Patient from Azerbaijan S.A. Limborska, A.N. Fedorov, V.L. Bukhman and M.I. Prosniak 197 The Gene of the Yeast Ribosomal Protein L32 M.D. Dabeva and J.R. Warner 203 Structural Comparison of some Microbial Ribonucleases C.P. Hill, G.G. Dodson, S.N. Borisova, A.G. Pavlovsky, K.M. Polyakov, B.V. Strokopytov and J. Sevcik 213 Structure Bases for Nucleotide Recognition by Guanyl specific Ribonucleases A.G. Pavlovsky, S.N. Borisova, B.V. Strokopytov, R.G. Sanishvili. A.A. Vagin and N.K. Chepurnova 217 Crystallization and Preliminary X-Ray Structural Studies of RNase Thl from Trichoderma harzianum K.M. Polyakov, B.V. Strokopytov, A.A. Vagin, S.I. Bezborodova and S.V. Shlyapnikov 223 Three-Dimensional Structure of RNase Cz from Aspergillus clavatus at 1.35 A Resolution K.M. Polyakov, B.V. Strokopytov, A.A. Vagin, S.I. Bezborodova and L. Orna 227 Amino Acid Composition and Influence of the Modification of some Amino Acid Residues on the Catalytic Activity of the Spleen Exonuclease A.T. Bakalova and L.B. Dolapchiev 233 Binding of the Metal Ions in the Active Site of the Exonuclease from Crotalus adamanteus Venom R.A. Vassileva and L.B. Dolapchiev 237 Ribosomal Nuclease with Activity Towards Double-Stranded RNA M.A. Siwecka, M. Rytel and J.W. Szarkowski' 245 Investigation of Immunoglobulin Light and Heavy Chain Genes Responsible for the Synthesis of Antibodies in Hybridoma PTF.02 S.M. Deyev, V.A. Ajalov, D.N. Urackov. A.G. Stepchenko, F. Franek and O.L. Polyanovsky 251 ix Regulation of Cytochrome P-450 Biosynthesis in Alkane Assimilating Yeast B. Wiedmann, M. Wiedmann, W.H. Schunck, S. Mauersberger. E. Kargel and H.G. MUller 259 On the Mechanism of Reutilization of Nuclear RNA Degradation Products: A Study in Vivo D.D. Genchev 267 Immunological Characterization of DNA-Dependent RNA Polymerase(s) of Spinach Chloroplasts E. Brautigam and S. Lerbs 275 DNA Crosslinked by UV Light to the Nuclear Lamina is Enriched in Pulse-Labeled Sequences Z.I. Galcheva-Gargova 283 The Mechanism of Arabinofuranosyl-Cytosine Inhibition in Undifferentiated Human B Lymphocytes T. Spasokukotskaja, J. Taljanidisz, M. Benczur and M. Staub 289 Closing of the Symposium by J. Zelinka, Corresponding Member of the Czechoslovak and Slovak Academy of Sciences, Director of the Institute of Molecular Biology, Slovak Academy of Sciences 297 Participants 299 Author Index 303 Subject Index 305 x DNA METHYLATION AND DNA METHYLTRANSFERASE IN WHEAT Hartmut Follmann. Roland Schleicher and J8rg Balzer Fachbereich Chemie. Abteilung Biochemie der Philipps UniversitAt D-3550 Marburg. Fed. Rep. Germany Plant DNA is distinguished from the deoxyribonucleic acid of all other eukaryotic organisms by its substantial amount of the modified base. 5- methylcytosine (mCyt). mCyt is not detectable in most fungi and in invert ebrates. it constitutes only up to 1% of the bases in vertebrate DNA. but it contributes 5-8 mol% of the total base composition in average plant DNA. Thus. one fifth to one third (20-35%) of the cytosine residues are modified in all plants. and nearly all cytosines are replaced by the methylated analog in some special plant DNA fractions. This unique base composition of plant DNA was recognized more than three decades ago [1]; however details of the distribution and formation of mCyt in the plant kingdom have received little attention until recently and specific functions are still unknown today. It is almost impossible to conceive that all these'modified cytosine residues could serve as built-in regulatory signals that determine gene inactivity or activity. the function which has been demonstrated in recent years for the few mCyt residues present in mammalian genes [2]. DNA methylation is a postreplicational event in which methyl groups are transferred from S-adenosylmethionine onto specific cytosine residues (mostly those in C-G sequences) of DNA; no cytosine modification occurs on the mononucleotide level. The reaction is catalyzed by DNA methyltrans ferases (EC 2.1.1.37) which have thus far been characterized almost exclu sively from mammalian sources. COOH COOH ~H-NH2 NH2 ~H-NH2 NNH)2 CH2 - N~CH3 CH2 CH2 O~N.!l CH2 oJ.-N + CH3-~-C~d.nin. I S-CH~d.nin. I ONA DNA Cytosine SAM OH OH 5 -Methylcytosi ne SAH OH OH We reasoned that the high amount of mCyt in plants requires an efficient enzyme system which might differ from the DNA methylase found in animal cells in activity and in specificity. and could thus provide insight . 1 into the origin and functions of DNA methylation in plants. With the exception of methylase activity in extracts from pea seedlings [3] and the enzyme purified from the unicellular algae, Chlamydomonas reinhardii [4] DNA methyltransferase has not been demonstrated in plants. Because the DNA of the green algae does not exhibit plant-specific mCyt level (0.7%) it was even uncertain whether the Chlamydomonas enzyme could be compared with that of higher plants at all. It is our aim to develop an in vitro system in which plant DNA methyl ation can be simulated qualitatively and quantitatively. To this aim we have purified to near homogeneity a highly active DNA methyltransferase from wheat embryo and initiated an analysis of the distribution of mCyt during wheat seed germination and in wheat DNA fractions of different sequence complexity. WHEAT DNA METHYLTRANSFERASE Germinating seeds are a better source than green tissues for .the characterization of the enzymes of nucleic acid metabolism in plants. DNA methylase activity in germinating wheat embryo had been shown to increase two- to threefold during and following the first round of DNA replication (i.e., 15-20 hours after the uptake of water) but the enzyme was also present in dry, ungerminated seeds [5]. Thus, unlike the enzyme of deoxy ribonucleotide biosynthesis [6], DNA methylase is not confined to the S (or G2) phase of a cell cycle. The preparation of intact cell nuclei from wheat embryo by Percoll density gradient centrifugation provided a basis for the purification of wheat DNA methyltransferase [7]. After separation of tightly bound endogenous DNA on a column of DEAE cellulose the enzyme was purified further by· chromatography on Sephadex G-75, Blue Sepharose, and DNA cellulose. This enzyme preparation had a specific activity of 2 nmo1 CHs incorporation·h-L.mg-l and was enriched 300-fold over the cell free tissue homogenate. It exhibited two protein bands on SDS poly acrylamide electrophoresis gels, corresponding to M = 50,000 and 35,000. Under native conditions, a molecular weight of 50,050 - 55,000 was estab lished by centrifugation in sucrose gradients. DNA methylase from maize seedlings could be obtained in a similar way. The properties of wheat DNA methyltransferase are compared with those of the enzyme from Chlamydomonas and of some mammalian proteins in Table 1. It is obvious that the enzymes isolated from a unicellular and a higher plant are similar, but differ strongly in molecular weight and in speci ficity from the mammalian enzymes. DNA methylation in plants vs. animals is not only characterized by a much higher level of methy1cytosine but also by lower sequence specificity Table 1. DNA Methy1transferases purified from mammalian and plant sources. spec.activity Source of enzyme "r specificity for DNA pmol.h-1.mg-1 ref. calf thymus 130 000 ss>ds, hetero>homologous 600 15 rat liver 115000 5 000 16 mouse ascites cells 180 000 1 500 17 human placenta 135 000 2 000 J8 Chlamydomonas reinhardii 58000 ds >55, homo = heterologous 180 4 wheat embryo 55 000 ds >55, homo > heterologous 2 000 7 2