Isolation, partial purification and characterization of phospholipase A2 from Naja Katiensis venom

The most effective and acceptable therapy for snakebite victims is the immediate administration of antivenin which is limited by problems of hypersensitivity reactions in some individuals and its inability to resolve the local effects of the venom. The aim of this study was to isolate, partially purify and characterize phospholipase A2 from Naja Katiensis venom. Phospholipase A2 was partially purified via a two-step process: gel filtration on Sephadex G-75 and ion exchange chromatography using CM Sephadex, and subjected to SDS-PAGE analysis. From the results, the specific activity of the partially purified PLA2 decreased from 0.67μmol/min/mg in crude venom to 0.29μmol/min/mg after ion exchange chromatography with a yield of 5% and purification fold of 0.43. The optimum temperature of the purified PLA2 was found to be 35ºC and optimum p.H of 7. velocity studies for the determination of kinetic constants using L-a-lecithin as substrate revealed a Km of 1.47mg/ml and Vmax of 3.32μ moles/min/mg. The sodium dodecyl sulphate polyacrylamide gel electrophoresis of the purified PLA2 showed a distinct band with molecular weight estimated to be 14KDa. In conclusion, the present study shows that phospholipase A2 was isolated, purified and characterized. This may serve as a promising candidate for future development of a novel anti-venin drug.

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Studies on an Inhibitor of Plasminogen Activation in Human Serum

Thrombosis and Haemostasis ◽

10.1055/s-0038-1649120 ◽

1973 ◽

Vol 30 (02) ◽

pp. 414-424 ◽

Cited By ~ 20

Author(s):

Ulla Hedner

Keyword(s):

Ion Exchange ◽

Human Serum ◽

Antithrombin Iii ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Specific Adsorption ◽

Partial Purification ◽

Plasminogen Activation ◽

Preparative Electrophoresis

SummaryA procedure is described for partial purification of an inhibitor of the activation of plasminogen by urokinase and streptokinase. The method involves specific adsorption of contammants, ion-exchange chromatography on DEAE-Sephadex, gel filtration on Sephadex G-200 and preparative electrophoresis. The inhibitor fraction contained no antiplasmin, no plasminogen, no α1-antitrypsin, no antithrombin-III and was shown not to be α2 M or inter-α-inhibitor. It contained traces of prothrombin and cerulo-plasmin. An antiserum against the inhibitor fraction capable of neutralising the inhibitor in serum was raised in rabbits.

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Purification of rabbit bone inhibitor of collagenase

Biochemical Journal ◽

10.1042/bj1950159 ◽

1981 ◽

Vol 195 (1) ◽

pp. 159-165 ◽

Cited By ~ 244

Author(s):

T E Cawston ◽

W A Galloway ◽

E Mercer ◽

G Murphy ◽

J J Reynolds

Keyword(s):

Tissue Culture ◽

Gel Electrophoresis ◽

Polyacrylamide Gel Electrophoresis ◽

Sodium Dodecyl ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Serine Proteinases ◽

Bacterial Collagenase ◽

Rabbit Bone

1. Rabbit bones in tissue culture synthesize an inhibitor of collagenase during the first 4 days of culture. 2. The inhibitor was purified by a combination of gel filtration, concanavalin A--Sepharose chromatography, ion-exchange chromatography and zinc-chelate affinity chromatography. 3. The purified inhibitor migrated as a single band on sodium dodecyl sulphate/polyacrylamide-gel electrophoresis and had a mol.wt. of 28000. 4. The inhibitor blocked the activity of the metalloproteinases collagenase, gelatinase, neutral proteinase III (proteoglycanase), human leucocyte collagenase and gelatinase, but not thermolysin or bacterial collagenase. The serine proteinases plasmin and trypsin were not inhibited. 5. The inhibitor interacted with purified rabbit bone collagenase with 1:1 stoichiometry. 6. The inhibitory activity was lost after incubation for 1 h at 90 degrees C, after treatment with trypsin (250 micrograms/ml) at 37 degrees C for 30 min and after reduction and alkylation.

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Isolation, in the intact state, of the pterin molybdenum cofactor from xanthine oxidase

Biochemical Journal ◽

10.1042/bj2630477 ◽

1989 ◽

Vol 263 (2) ◽

pp. 477-483 ◽

Cited By ~ 10

Author(s):

J Deistung ◽

R C Bray

Keyword(s):

Aqueous Solution ◽

Ion Exchange ◽

Xanthine Oxidase ◽

Specific Activity ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Molybdenum Cofactor ◽

Anaerobic Conditions ◽

Intact State

A procedure is described for isolation of the pterin molybdenum cofactor, in the active molybdenum-containing state, starting from purified milk xanthine oxidase. The method depends on the use of anaerobic-glove-cabinet techniques and on working in aqueous solution, in the presence of 1 mM-Na2S2O4. SDS was used to denature the protein, followed by ion-exchange chromatography and gel filtration. The cofactor, obtained at concentrations up to 0.5-1.0 mM, was fully active in the nit-1 assay [Hawkes & Bray (1984) Biochem. J. 214, 481-493], with a specific activity of 22 nmol of NO2-/min per pg-atom of Mo (with 15% molybdate-dependence). The Mr, determined by gel filtration, was about 610, consistent with the structure proposed by Kramer, Johnson, Ribeiro, Millington & Rajagopalan [(1987) J. Biol. Chem. 262, 16357-16363]. At pH 5.9, under anaerobic conditions, the cofactor was stable for at least 300 h at 20-25 degrees C.

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Partial purification of two lithocholic acid-binding proteins from rat liver 100000g supernatants

Biochemical Journal ◽

10.1042/bj1650425 ◽

1977 ◽

Vol 165 (3) ◽

pp. 425-429 ◽

Cited By ~ 29

Author(s):

R C Strange ◽

R Cramb ◽

J D Hayes ◽

I W Percy-Robb

Keyword(s):

Ion Exchange ◽

Binding Proteins ◽

Lithocholic Acid ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Anion Binding ◽

Partial Purification ◽

Transferase Activity ◽

Glutathione S Transferase

1. The partial purification of two lithocholic acid-binding proteins from liver 100 000g supernatants is described. 2. Gel-filtration, (NH4)2SO4 fractionation, Ca3(PO4)2 fractionation and ion-exchange chromatography were used. 3. Both proteins exhibited glutathione S-transferase activity; one may be the non-specific anion-binding protein ligandin. 4. Glutathione S-transferase activity of one of the binding proteins was inhibited by lithocholic acid.

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Dephosphorylation of Phytate by Using theAspergillus niger Phytase with a High Affinity for Phytate

Applied and Environmental Microbiology ◽

10.1128/aem.65.10.4682-4684.1999 ◽

1999 ◽

Vol 65 (10) ◽

pp. 4682-4684 ◽

Cited By ~ 31

Author(s):

Tadashi Nagashima ◽

Tatsuya Tange ◽

Hideharu Anazawa

Keyword(s):

Phytic Acid ◽

Polyacrylamide Gel Electrophoresis ◽

Sodium Dodecyl ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Aspergillus Ficuum ◽

Michaelis Constant ◽

High Affinity ◽

Significant Difference

ABSTRACT A phytase (EC 3.1.3.8 ) with a high affinity for phytic acid was found in Aspergillus niger SK-57 and purified to homogeneity in four steps by using ion-exchange chromatography (two types), gel filtration, and chromatofocusing. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis of the purified enzyme gave a single stained band at a molecular mass of approximately 60 kDa. The Michaelis constant of the enzyme for phytic acid (18.7 ± 4.6 μM) was statistically analyzed. In regard to the orthophosphate released from phytic acid, a significant difference between a lowKm phytase from A. niger SK-57 and a high Km phytase from Aspergillus ficuum was recognized.

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Multiplicity of extracellular β-(1,4)-endoglucanases of Bacteroides succinogenes S85

Canadian Journal of Microbiology ◽

10.1139/m84-146 ◽

1984 ◽

Vol 30 (7) ◽

pp. 930-937 ◽

Cited By ~ 17

Author(s):

H. E. Schellhorn ◽

C. W. Forsberg

Keyword(s):

Ion Exchange ◽

Microcrystalline Cellulose ◽

Polyacrylamide Gel Electrophoresis ◽

Gel Filtration ◽

Glucose Production ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Reducing Sugar ◽

Sugar Production ◽

Endoglucanase Activity

During growth on 0.2% (w/v) microcrystalline cellulose, Bacteroides succinogenes S85 produces endoglucanase activity which can be separated by centrifugation into sedimentable and nonsedimentable fractions. The sedimentable activity, after solubilization with Triton X-100, was resolved into four components by ion-exchange chromatography and these were further fractionated by nondenaturing polyacrylamide gel electrophoresis (PAGE). The nonsedimentable activity contained three enzymic components as determined by gel filtration. Like the preparations derived from the sedimentable fraction, these components yielded a multiplicity of endoglucanases when electrophoresed under nondenaturing conditions. The fractions obtained by ion-exchange chromatography and by gel filtration were assayed for endoglucanase activity by both viscometric assays and reducing sugar production using carboxymethylcellulose as the substrate. Plots of the fluidity change in the enzyme–substrate preparation in relation to reducing sugar production revealed the presence of two distinct groups of endoglucanases differing in catalytic activity. Two of the components from the nonsedimentable fraction had more exoglucanase-like activity than either the third nonsedimentable fraction or any of the four fractions derived from the sedimentable material. These two enzymes could be further differentiated on the basis of glucose production from microcrystalline cellulose and by their relative activity toward p-nitrophenyl cellobioside, a chromogenic substrate.

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Purification, characterization, and antifungal activity of chitinase from Fusarium chlamydosporum, a mycoparasiteto groundnut rust, Puccinia arachidis

Canadian Journal of Microbiology ◽

10.1139/w98-043 ◽

1998 ◽

Vol 44 (7) ◽

pp. 646-651 ◽

Cited By ~ 28

Author(s):

N Mathivanan ◽

V Kabilan ◽

K Murugesan

Keyword(s):

Gel Electrophoresis ◽

Polyacrylamide Gel Electrophoresis ◽

Sodium Dodecyl ◽

Gel Filtration ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Puccinia Arachidis ◽

Fusarium Chlamydosporum ◽

Groundnut Rust ◽

Germ Tubes

Chitinase (EC 3.2.1.14) was isolated from the culture filtrate of Fusarium chlamydosporum and purified by ion-exchange chromatography and gel filtration. The molecular mass of purified chitinase was 40 kDa as estimated by sodium dodecyl sulfate polyacrylamide gel electrophoresis. Chitinase was optimally active at a pH of 5 and stable from pH 4 to 6 and up to 40°C. Among the metals and inhibitors tested, mercuric chloride completely inhibited the enzyme activity. The activity of chitinase was high on colloidal and pure chitin. The purified chitinase inhibited the germination of uredospores of Puccinia arachidis and also lysed the walls of uredospores and germ tubes. The results from these experiments indicated that chitinase of F. chlamydosporum plays an important role in the biocontrol of groundnut rust. Key words: Fusarium chlamydosporum, chitinase, purification, Puccinia arachidis, uredospores.

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Purification and Partial Characterization of a Murein Hydrolase, Millericin B, Produced by Streptococcus milleri NMSCC 061

Applied and Environmental Microbiology ◽

10.1128/aem.66.1.23-28.2000 ◽

2000 ◽

Vol 66 (1) ◽

pp. 23-28 ◽

Cited By ~ 38

Author(s):

M. Beukes ◽

G. Bierbaum ◽

H.-G. Sahl ◽

J. W. Hastings

Keyword(s):

Ion Exchange ◽

Specific Activity ◽

Gel Filtration ◽

Fold Increase ◽

Ion Exchange Chromatography ◽

Exchange Chromatography ◽

Amino Acid Sequences ◽

Antimicrobial Substances ◽

Streptococcus Milleri ◽

N Terminus

ABSTRACT Streptococcus milleri NMSCC 061 was screened for antimicrobial substances and shown to produce a bacteriolytic cell wall hydrolase, termed millericin B. The enzyme was purified to homogeneity by a four-step purification procedure that consisted of ammonium sulfate precipitation followed by gel filtration, ultrafiltration, and ion-exchange chromatography. The yield following ion-exchange chromatography was 6.4%, with a greater-than-2,000-fold increase in specific activity. The molecular weight of the enzyme was 28,924 as determined by electrospray mass spectrometry. The amino acid sequences of both the N terminus of the enzyme (NH2 SENDFSLAMVSN) and an internal fragment which was generated by cyanogen bromide cleavage (NH2 SIQTNAPWGL) were determined by automated Edman degradation. Millericin B displayed a broad spectrum of activity against gram-positive bacteria but was not active againstBacillus subtilis W23 or Escherichia coli ATCC 486 or against the producer strain itself. N-Dinitrophenyl derivatization and hydrazine hydrolysis of free amino and free carboxyl groups liberated from peptidoglycan digested with millericin B followed by thin-layer chromatography showed millericin B to be an endopeptidase with multiple activities. It cleaves the stem peptide at the N terminus of glutamic acid as well as the N terminus of the last residue in the interpeptide cross-link of susceptible strains.

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Purified Factor XII Has a Higher Specific Activity than the Parent Molecule in Plasma

Thrombosis and Haemostasis ◽

10.1055/s-0038-1647478 ◽

1991 ◽

Vol 65 (02) ◽

pp. 169-173 ◽

Cited By ~ 3

Author(s):

Walter A Wuillemin ◽

Miha Furlan ◽

Isabella Huber ◽

Bernhard Lämmle

Keyword(s):

Specific Activity ◽

Polyacrylamide Gel Electrophoresis ◽

Sodium Dodecyl ◽

Gel Filtration ◽

Anion Exchange Chromatography ◽

Exchange Chromatography ◽

Factor Xii ◽

Parent Molecule ◽

Proteolytic Activation ◽

Filtration Step

SummaryThe specific clot promoting activity of factor XII (F XII) in plasma samples from 50 healthy adults was between 30 and 48 U/ mg, whereas the specific activity of purified F XII ranged from 55 to 66 U/mg. This difference was neither due to partial proteolytic activation during purification of F XII nor to the influence of plasma protease inhibitors. Purified F XII showed normal size and charge, as demonstrated by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and isoelectric focusing, respectively. The increase of the specific F XII activity during the purification process mainly occurred after anion exchange chromatography on DEAE-Sephadex and after the final gel filtration step. Upon dextran sulfate activation, proteolytic cleavage of F XII and generation of kallikrein-like amidolytic activity was faster in F XII deficient plasma containing purified F XII than in F XII deficient plasma containing a corresponding amount of pooled normal plasma (NHP). The binding to kaolin was similar for both, purified F XII and plasma F XII.In conclusion, purification alters the properties of F XII in an unknown way, resulting in an increased specific clot promoting activity.

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Purification and characterization of a phospholipase A2 from the venom of the coral snake, Micrurus fulvius microgalbineus (Brown and Smith)

Biochemical Journal ◽

10.1042/bj1790603 ◽

1979 ◽

Vol 179 (3) ◽

pp. 603-606 ◽

Cited By ~ 13

Author(s):

L D Possani ◽

A C Alagòn ◽

P L Fletcher ◽

M J Varela ◽

J Z Juliá

Keyword(s):

Amino Acid ◽

Phospholipase A2 ◽

Gel Electrophoresis ◽

Specific Activity ◽

Polyacrylamide Gel Electrophoresis ◽

Sodium Dodecyl ◽

Polyacrylamide Gel ◽

Coral Snake ◽

Phospholipase Activity ◽

Crude Venom

A phospholipase A2 was purified from the Mexican coral snake Micrurus fulvius microgalbieus (Brown and Smith). Gel filtration of the soluble crude venom on Sephadex g-50 resolved five fractions, of which fraction II had 98% of the total phospholipase activity. This fraction was rechromatographed on a CM-cellulose column that resolved eight fractions, four of which had an important phospholipase activity. The first fraction (II-1) was homogeneous by polyacrylamide-gel electrophoresis and displayed a phospholipase specific activity of 920 units/mg of protein. The apparent molecular weight as determined by sodium dodecyl sulphate/polyacrylamide-gel electrophoresis was approx. 14000. The amino acid analysis revealed the presence of 119 amino acid residues, with 12 half-cystines. the N-terminal sequence was shown to be Ser-Leu-Leu-Asx-Phe-Lys-Asx-Met-Ile-Glu-Ser-Thr..., which is homologous with that of phospholipases from other snake venoms.

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