First determination of the isozyme patterns of phosphoglycerate mutases (E.C.2.7.5.3) and phosphoglycerate kinases (E.C.2.7.2.3) in human tissues.

We present in this paper the first report about identification of several fractions of phosphoglycerate mutase (PGlyM) activity using starch gel electrophoresis and two different buffer systems. A typical muscle form of PGlyM was detected. It is also shown that isozymes of phosphoglycerate kinase (PGK) can be separated through the buffer system used by Spencer et al; (1964) for the phosphogluco mutase.     

Multiple forms of enolase (E.C. 4.2.1.11): their distribution in human tissues.

By means of starch gel electrophoresis, the enzyme enolase was found to be a family of at least 3 isozymes in human tissues. Enolase III shows a strong band in extracts of human brain and in some malignant tumors.     

Isozyme variations in acetaldehyde dehydrogenase (E.C.1.2.1.3) in human tissues

Summary NAD-dependent acetaldehyde dehydrogenase (ALDH) of human tissues was investigated by electrophoresis and enzyme assay. ALDH is located mainly in the liver and kidney. The isozymes consist of at least six different components. Five different phenotypes were found in a total of 68 human liver and kidney specimens. It is likely that three isozyme sets are concerned in determining ALDH types. The distribution of various phenotypes of ALDH isozyme sets is presented.     

Gene frequency of delta-aminolevulinate dehydratase (E.C. 4.2.1.24) in a West German population

The delta-aminolevulinate dehydrase (E.C. 4.2.1.24) gene frequencies were investigated by starch gel electrophoresis in 711 unrelated individuals from the Düsseldorf area. The following gene frequencies were found: ALADH1 0.929, ALADH2 0.071. The frequency reported for ALADH1 is only slightly higher than that for Italy.     

Purification and characterization of an endonuclease (E.C. 3.1.30.1) from Streptomyces tendae

A single-strand-specific endonuclease which converted negatively supercoiled DNA to open-circular and linear DNA was purified to homogeneity with Hb-Sepharose 4B, DEAE Trisacryl M, HA-Ultrogel and PBE-94 chromatofocusing from extracts of Streptomyces tendae ATCC 31160. Bio-Gel P-200 chromatography and electrophoresis in SDS-PAGE indicated the native protein was a monomer with a molecular weight of approximately 40-kDa. This enzyme did not hydrolyze double-stranded linear DNA but digested RNA and circular single-strand DNA. Sequence specificity for nicking of negatively supercoiled DNA was not detected.     

Genetic variants of glucose phosphate isomerase (E.C. 5.3.1.9) in canine erythrocytes

Genetic polymorphism of glucose phosphate isomerase (GPI) was found in the erythrocytes of dogs of six Japanese breeds by using starch gel electrophoresis. Analysis of parentage records of dogs revealed that the phenotypic variation of erythrocyte glucose phosphate isomerase was controlled by one autosomal locus with two codominant alleles, GPIA and GPIB. The allele GPIB was observed in the following breeds: San'in-Shiba, Shinshu-Shiba, Shikoku, Kai and Kishu, but not in Hokkaidoes and Akitas. All the dogs belonging to 25 European breeds, 5 oriental or China-origin (except Japan) breeds examined in this experiments had the genotype constitution GPIA/GPIA, whereas one Dalmation dog was heterozygous GPIA/GPIB.     

Extracellular alpha galactosidase (E.C. 3.2.1.22) from Aspergillus ficuum NRRL 3135 purification and characterization

Extracellular alpha-galactosidase, a glycoprotein from the extracellular culture fluid of Aspergillus ficuum grown on glucose and raffinose in a batch culture system, was purified to homogeneity in five steps by ion exchange and hydrophobic interaction chromatography. The molecular mass of the enzyme was 70.8 Kd by SDS polyacrylamide gel electrophoresis and 74.1 Kd by gel permeation HPLC. On the basis of a molecular mass of 70.7 Kd, the molar extinction coefficient of the enzyme at 279 nm was estimated to be 6.1 X10(4) M-1 cm-1. The purified enzyme was remarkably stable at 0 degrees C. It had a broad temperature optimum and maximum catalytic activity was at 60 degrees C. It retained 33% of its activity after 10 min. at 65 degrees C. It had a pH optimum of 6.0. It retained 62% of its activity after 12 hours at pH 2.3. The Kms for p-nitrophenyl-alpha-D-galactopyranoside, o-nitrophenyl-alpha-D-galactopyranoside and m-nitrophenyl-alpha-D-galactopyranoside are: 1462, 839 and 718 microM. The enzyme was competitively inhibited by mercury (19.8 microM), silver (21.5 microM), copper (0.48 mM), zinc (0.11 mM), galactose (64.0 mM) and fructose (60.3 mM). It was inhibited non-competitively by glucose (83.2 mM) and uncompetitively by mannose (6.7 mM).     

Genetic polymorphism of delta-aminolaevulinic acid dehydratase (E.C. 4.2.1.24, ALAD) in the domestic rabbit

A genetic polymorphism of delta-aminolaevulinic acid dehydratase (ALAD) in the domestic rabbit, Oryctolagus cuniculus, was detected by starch gel electrophoresis. Family data (15 matings with 49 offspring) support the genetic model of two common codominant alleles at an autosomal locus. Gene frequencies were calculated in a random sample of 55 mixed breed, unrelated domestic rabbits: ALAD1 = 0.31 and ALAD2 = 0.69.     

Extracellular phytase (E.C. 3.1.3.8) from Aspergillus ficuum NRRL 3135: purification and characterization

Extracellular phytase from Aspergillus ficuum, a glycoprotein, was purified to homogeneity in 3 column chromatographic steps using ion exchange and chromatofocusing. Results of gel filtration chromatography and SDS-polyacrylamide gel electrophoresis indicated the approximate molecular weight of the native protein to be 85-100-KDa. On the basis of a molecular weight of 85-KDa, the molar extinction coefficient of the enzyme at 280 nm was estimated to be 1.2 X 10(4) M-1 cm-1. The isoelectric point of the enzyme, as deduced by chromatofocusing, was about 4.5. The purified enzyme is remarkably stable at 0 degree C. Thermal inactivation studies have shown that the enzyme retained 40% of its activity after being subjected to 68 degrees C for 10 minutes, and the enzyme exhibited a broad temperature optimum with maximum catalytic activity at 58 degrees C. The Km of the enzyme for phytate and p-nitrophenylphosphate is about 40 uM and 265 uM, respectively, with an estimated turnover number of the enzyme for phytate of 220 per sec. Enzymatic deglycosylation of phytase by Endoglycosidase H lowered the molecular weight of native enzyme from 85-100-KDa to about 76-KDa; the digested phytase still retained some carbohydrate as judged by positive periodic acid-Schiff reagent staining of the electrophoresed protein. Immunoblotting of the phytase with monoclonal antibody 7H10 raised against purified native enzyme recognized not only native but also partially deglycosylated protein.     

Mitochondrial malic enzyme (E.C. 1.1.1.40) in human leukocytes: Formal genetics and population genetics

Summary Mitochondrial malic enzyme ME_M (E.C. 1.1.1.40) is present in human leukocytes; the polymorphism of ME_M thus can be easily demonstrated using routine starch gel electrophoresis. Data on formal genetics are given. The gene frequency of ME ₁ ^M was estimated to be 0.67±0.02.     

Extracellular Phytase (E. C. 3.1.3.8) from Aspergillus Ficuum NRRL 3135: Purification and Characterization

Extracellular phytase from Aspergillus ficuum, a glycoprotein, was purified to homogeneity in 3 column chromatographic steps using ion exchange and chromatofocusing. Results of gel filtration chromatography and SDS-polyacrylamide gel electrophoresis indicated the approximate molecular weight of the native protein to be 85–100-KDa. On the basis of a molecular weight of 85–KDa, the molar extinction coefficient of the enzyme at 280 nm was estimated to be 1.2 × 10⁴ M-l cm-1. The isoelectric point of the enzyme, as deduced by chromatofocusing, was about 4.5. The purified enzyme is remarkably stable at 0°C. Thermal inactivation studies have shown that the enzyme retained 40% of its activity after being subjected to 68°C for 10 minutes, and the enzyme exhibited a broad temperature optimum with maximum catalytic activity at 58°C. The Km of the enzyme for phytate and p-nitrophenylphosphate is about 40 uM and 265 uM, respectively, with an estimated turnover number of the enzyme for phytate of 220 per sec. Enzymatic deglycosylation of phytase by Endoglycosidase H lowered the molecular weight of native enzyme from 85–100-KDa to about 76–KDa; the digested phytase still retained some carbohydrate as judged by positive periodic acid-Schiff reagent staining of the electrophoresed protein. Immunoblotting of the phytase with monoclonal antibody 7H10 raised against purified native enzyme recognized not only native but also partially deglycosylated protein.     

Polymorphism of alanine aminotransferase (E.C.2.7.6.1): Common and rare alleles

Summary Gene frequencies of common and rare GPT alleles derived from an investigation of 1139 unrelated, healthy individuals from southwestern Germany are given. GPT typing was performed by means of horizontal starch gel electrophoresis in a Tris-histidinexHCl buffer system. In addition, a new electrophoretic variant, GPT ⁹, is described.The frequencies of the GPT alleles observed were calculated as: GPT ¹ 0.4987; GPT ², 0.4686; GPT ^1M, 0.022; GPT ⁰, 0.005; GPT ³, 0.0022; GPT ⁴, 0.0025; GPT ⁸, 0.0005; GPT ⁹, 0.0005.     

Genetic polymorphism of glycerol-3-phosphate dehydrogenase (E.C.: 1.1.1.8)

Summary By means of starchgel electrophoresis several distinct proteins with G-3-PD activity can be detected in Primates. The relative activities of these isoenzymes are found to vary markedly from tissue to tissue. It is presumed that the G-3-PD proteins are dimers composed of two nonidentical polypeptide subunits (chain A and B), which are determined by two separate gene loci (G-3-PD _A and G-3-PD _B). In liver, kidney and skeletal muscle the subunit B is in great excess, while in heart and brain both subunits A and B are present in almost equal proportions. It is concluded, that the various isozyme patterns are the consequence of random combinations of different polypeptide chains. The results obtained so far indicate, that in Primates 2 alleles occur at the G-3-PD _A locus and 5 alleles at the G-3-PD _B locus. Formal notations are given, and a study on population genetics is reported.

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Zusammenfassung Bei den Primaten können mit der Stärkegelelektrophorese verschiedene G-3-PD-aktive Proteine nachgewiesen werden. Die transspezifische Variabilität ist beträchtlich. Für eine formalgenetische Interpretation ist das Modell zu unterlegen: zwie Cistrons G-3-PD _A und G-3-PD _B mit Information für G-3-PD-Polypeptidketten. Homozygote Individuen besitzen 3 Isoenzymbanden, da die beiden Polypeptidketten zu Dimermolekülen frei assoziieren. Heterozygote Individuen für das Cistron G-3-PD _A bzw. G-3-PD _B besitzen jeweils 6 Isoenzymbanden. Bei doppelt heterozygoten Individuen (sowohl für das Cistron G-3-PD _A als auch für G-3-PD _B) sind insgesamt 10 Isoenzymbanden zu erwarten. Unterschiede in den Syntheseraten für A- und B-Polypeptidketten bedingen eine stark ausgeprägte organspezifische Variabilität. In Leber, Niere und skeletmuskel überwiegt die Synthese für B-Ketten, im Herzmuskel und Gehirn werden A- und B-Ketten in annähernd gleicher Menge gebildet. Auf Grund der bisher vorliegenden Ergebnisse ist bei den Primaten mit 2 allelischen Varianten für das Cistron G-3-PD _A und mit 5 allelischen Varianten für das Cistron G-3-PD _B zu rechnen.

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(Director: Prof. Dr. Dr. H. Ritter)

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Supported by the Deutsche Forschungsgemeinschaft.     

Structure of enoate reductase from a Clostridium tyrobutyricum (C. spec. La1)

Enoate reductase from Clostridium tyrobutyricum was purified by a rapid novel procedure. Chromatography on DEAE-Sepharose and on hydroxyapatite resulted in a high yield of about 90% pure enzyme in less than 10 h. A purity greater than 98% could be obtained by additional chromatography on Sephacryl S-300. The enzyme sediments in the analytical ultracentrifuge as a single, symmetrical boundary with a velocity of S(0)20,w = 24.9 S. Equilibrium ultracentrifugation yielded a molecular mass of 940 000 +/- 20 000 Da. The enzyme contains one type of subunit as shown by dodecyl sulfate electrophoresis and partial sequence determination. A subunit molecular mass of about 73 000 Da was established by dodecyl sulfate electrophoresis and by sedimentation equilibrium analysis in guanidine hydrochloride. In addition to FAD, iron and labile sulfur, the enzyme purified by the new method showed approximately 0.7 mol of FMN per mol of subunit. A dissociation product sedimenting at a velocity of S(0)20,w = 9.8 S can be obtained by various experimental protocols. The fragment was obtained in pure form by gel permeation chromatography. The molecular mass was 230 000 +/- 10 000 Da as shown by sedimentation equilibrium analysis. Thus it appears that the dissociation product is a trimer of the 73 000-Da subunit. The formation of the 10-S fragment by dissociation of the native enzyme is accompanied by the loss of most of the FMN, whereas the FAD content is not changed. The fragment catalysed the reduction of acetylpyridine adenine dinucleotide by NADH. However, enoate reductase activity with NADH or methylviologen as cosubstrate was low. Electron micrographs of negatively stained enoate reductase show trigonal symmetry. The data suggest that enoate reductase is a dodecamer (tetramer of trimers) with tetrahedral symmetry.     

Genetic variants of glucose phosphate isomerase (E.C. 5.3.1.9) in canine erythrocytes*

Genetic polymorphism of glucose phosphate isomerase (GPI) was found in the erythrocytes of dogs of six Japanese breeds by using starch gel electrophoresis. Analysis of parentage records of dogs revealed that the phenotypic variation of erythrocyte glucose phosphate isomerase was controlled by one autosomal locus with two codominant alleles, GPI^Aand GPI^B. The allele GPI^Bwas observed in the following breeds: San'in-Shiba, Shinshu-Shiba, Shikoku, Kai and Kishu, but not in Hokkaidoes and Akitas. All the dogs belonging to 25 European breeds, 5 oriental or China-origin (except Japan) breeds examined in this experiments had the genotype constitution GPI^A/GPI^A, whereas one Dalmation dog was heterozygous GPI^A/GPI^B.     

补体C3与BPI活性区融合蛋白（CB）的构建与表达

补体C3和杀菌通透性增加蛋白（BPI）对血液中的病原体均有黏附、促吞噬甚至杀灭作用,但两者的作用机制不同,制备两者活性区融合蛋白,可能具有更好的清除血液病原的作用。通过重叠延伸PCR融合人补体C3的补体受体Ⅰ、Ⅲ两个结合区,同时调取了杀菌通透性增加蛋白（BPI）活性区段rBPI,先后将补体C3活性区与BPI蛋白功能区基因克隆入原核表达载体pET28a中,获得融合蛋白（CB）表达载体pET28-CB,在大肠杆菌中进行了高表达产量、可溶性表达等条件的摸索,CB融合蛋白主要以包涵体形式表达,Western印迹证明CB具有C3的抗原活性,将包涵体蛋白变性与复性后,利用Ni2+固相化的螯合Sepharose Fast Flow亲和层析柱进行浓缩和纯化,最后得到了纯度较高的CB原核表达蛋白。CB融合蛋白的构建和高效表达、纯化为下步探讨其在促进血液病原清除上的功能鉴定和应用奠定了基础。     

The Studies of the Stabilizing Factor of the Nitrate Reductase(E. C. 1.6.6.2) Activity from the Tomato(Lycopersicum esculentum)Leaves

A stabilizing factor of NR activity was isolated from tomato leaf homogenate by (NH4)2SO4 precipitation, boiling water treatment, Sephadex G-75 column and DEAE 52 column and dialysis against water. This factor appeared as band on polyacryl amide gel electrophoresis. This factor protected NR activity of tomato leaves from inactivation by temperature. It delayed the inactivation of N-R activity in wheat seedlings. when mixed with stabilizing factor and stored at 0 ℃ for nine days NR from wheat seedlings still kept its activity; without stabilizing factor, its activity was lost completely. Stabilizing factors both treated in boiling water in the process of isolation and isolated below 4 ℃ could stabilize and increase NR activity of tomato leaves. This factor existed in two forms, one free and one combined with some protein. It could be separated from the protein by heating during extraction. The stabilizing factor is different from FAD, haem, and proline.     

Determination of isozymes of phosphoglycerate-mutase (E.C.2.7.5.3) and enolase (E.C.4.2.1.11) in human erythrocytes.

525 human hemolysates were tested for the isozymic patterns of phosphoglycerate mutase and enolase. Genetic models for interpreting the pherograms are suggested.     

Purification and some properties of phospholipase C (alpha-toxin) of Clostridium perfringens.

1. Phospholipase C[EC 3.1.4.3] was purified from the culture filtrate of Clostridium perfringens by successive chromatographies on CM-Sephadex, DEAE-Sephadex, and Sephadex G-100. During the purification it was noted that, beside the monomer form of the enzyme which was purified, a part of the enzyme existed in active polymerized forms. 2. The purified preparation gave a single band on polyacrylamide gel electrophoresis and gave a single precipitin line in immunodiffusion with the National Standard gas gangrene (C. perfringens) antitoxin, indicating the homogeneity of the preparation. 3. The specific lecithin-hydrolyzing activity of the purified preparation was comparable to that of a preparation obtained by affinity chromatography, which had the highest specific activity previously reported. 4. The molecular weight of the purified enzyme was estimated to be 43,000 by SDS-polyacryl-amide gel electrophoresis, although the same preparation gave a molecular weight of 31,000 as determined by gel filtration on Sephadex G-150. From this and the above finding that a part of the enzyme exists in active polymerized forms, the discrepancy among reported values for the molecular weight of C. perfringens phospholipase C can be accounted for. 5. For maximum hydrolytic activity toward lecithin, the enzyme required sodium deoxycholate (SDC) and Ca2+ ions. In the presence of 6 mM Ca2+, the optimal molar ratio of SDC to lecithin for maximal hydrolytic activity was about 0.5 for dipalmitoyl lecithin and about 1.0 for egg lecithin. The effects of various divalent cations on the enzymatic hydrolysis were also investigated. 6. The effects of sodium deoxycholate and Ca2+ ions on the enzymatic hydrolysis are discussed, based on their possible roles in mixed micelle formation.     

Assignment of a gene for tryptophanyl-transfer ribonucleic acid synthetase (E.C. 6.1.1.2) to human chromosome 14

We describe a simple method for locating tryptophanyl-tRNA synthetase (E.C. 6.1.1.2) on cellulose acetate gels (Cellogel) following electrophoresis. Employing electrophoretic conditions which result in the separation of mouse and human tryptophanyl-tRNA synthetases, we have analyzed extracts of a number of independently derived mouse-human somatic cell hybrids and subclones derived from these hybrids for the presence of human tryptophanyl-tRNA synthetase. Electrophoretic patterns of hybrid extracts which contain human tryptophanyl-tRNA synthetase exhibit three bands. This is consistent with published evidence that the enzyme from mammalian cells is a homologous dimer. The electrophoretic patterns derived from some hybrids are unusual in that the human and hybrid bands of activity are more intense than the mouse band from the same hybrid. An analysis of hybrid cells and extracts indicates that human tryptophanyl-tRNA synthetase segregates with human chromosome 14 and with the only enzyme marker which has previously been assigned to this chromosome, nucleoside phosphorylase.R. M. D. was supported by a postdoctoral fellowship from the Damon Runyon Fund for Cancer Research. The work described was supported in part by grants from Cancer Research Campaign, the Medical Research Council, and NATO.