Your search keyword '"Plasminogen chemistry"' showing total 7 results

1. [Development and optimization of the methods for determining activity of plasminogen activator inhibitor-1 in plasma].

Author

Roka-Moĭia IaM, Zhernosiekov DD, Kondratiuk AS, and Hrynenko TV

Subjects

Animals, Cattle, Cyanogen Bromide chemistry, Fibrin chemistry, Fibrinogen chemistry, Fibrinolysin chemistry, Humans, Kinetics, Plasminogen chemistry, Tissue Plasminogen Activator chemistry, Biological Assay, Plasminogen Activator Inhibitor 1 blood

Abstract

The activity and content of plasminogen activator inhibitor-1 (PAI-1) are important indicators of pathological processes, because its content in plasma increases at acute myocardium infarction, tumor, diabetes mellitus, etc. The present work is dedicated to the development and optimization of the methods of PAI-1 activity definition, which can be used in clinical practice. We have proposed the modification of the method COATEST PAI with the usage of chromogenic substrate S2251. According to our modification, the cyanogen bromide fragments of human fibrinogen have been changed into bovine desAB-fibrin. We have also developed the method with the usage of fibrin films. In this method fibrin is used as a stimulator of activation reaction and as a substrate at the same time. Using fibrin, the native substrate of plasmin, we provide high specificity of the reaction and exclude the cross-reaction with other plasma enzymes.

Published

2013

2. [Regulation with alpha-2-antiplasmin of Glu-plasminogen activation by tissue activator on fibrin].

Author

Hrynenko TV, Zadorozhna MB, and Iusova OI

Subjects

Aminocaproic Acid chemistry, Animals, Cattle, Fibrin physiology, Humans, In Vitro Techniques, Models, Biological, Plasminogen physiology, Tissue Plasminogen Activator physiology, alpha-2-Antiplasmin physiology, Fibrin chemistry, Plasminogen chemistry, Tissue Plasminogen Activator chemistry, alpha-2-Antiplasmin chemistry

Abstract

Interaction of tissue plasminogen activator with alpha-2-antiplasmin and its influence on tissue activator binding to fibrin was studied. Alpha-2-Antiplasmin decreases the binding of tissue activator to fibrin by 20%. The inhibitor formed a complex with tissue plasminogen activator (Kd 78.2 nM) and had no effect on amidolytic activity of the activator. The tissue activator binding to alpha-2-antiplasmin decreases by 20-35% in the presence of 6-aminohexanoic acid. It indicates that not only kringle 2 of the tissue activator molecule takes part in complex formation with alpha-2-antiplasmin, but also other activator domains. Two models were proposed to explain the alpha-2-antiplasmin effect on the Glu-plasminogen activation by tissue activator on fibrin. In the first place, the inhibitor binds to fibrin in the site where the activator complex is localized. It can create steric hindrances for the proenzyme interaction with its activator on fibrin. In the second place, alpha-2-antiplasmin in a complex with tissue plasminogen activator can bring to a change in the activator conformation and a decrease of its functional activity.

Published

2006

3. [Inhibition of the process of Glu-plasminogen activation by tissue activator with fibrin, DDE-complex, and D-dimer using alpha-2-antiplasmin].

Author

Hrynenko TV, Zadorozhna MB, Platonova TM, and Volkov HL

Subjects

Animals, Cattle, Fibrinolysis, Humans, Kinetics, Time Factors, Fibrin chemistry, Fibrin Fibrinogen Degradation Products chemistry, Peptide Fragments chemistry, Plasminogen chemistry, Tissue Plasminogen Activator chemistry, alpha-2-Antiplasmin chemistry

Abstract

The alpha-2-antiplasmin influence on the Glu-plasminogen activation by tissue activator both on fibrin and fibrin(ogen) fragments was investigated. The kinetics of activation was studied and velocity of this process in the absence and presence of the inhibitor was calculated. It was established that alpha-2-antiplasmin decreased the velocity of Glu-plasminogen activation on desAABBfibrin, DDE-complex and DD-dimer and did no influence upon proenzyme activation on fibrinogen fragment--Ho1-DSK. In the presence of fibrin plasminogen activation linear related to the amount added tissue activator in limit concentration from 5 before 50 units/ml. It was shown that alpha-2-antiplasmin reduced the activation velocity with used concentration of tissue activator. Fibrin hydrolysis by plasmin, forming on its surface during the plasminogen activation by tissue activator, was also inhibited with alpha-2-antiplasmin. The obtained results are explained by the influence of the inhibitor on formation of the triple complex between plasminogen, tissue activator and fibrin, and competition of the alpha-2-antiplasmin for lysine-binding sites of tissue activator kringle 2 or for binding sites of the activator on fibrin.

Published

2005

4. [Degradation of streptokinase and the catalytic properties of the plasmin-streptokinase complex].

Author

Hrynenko TV, Makohonenko IeM, Iusova OI, and Cederholm-Williams SA

Subjects

Catalysis, Enzyme Stability, Fibrinolysis drug effects, Humans, Kinetics, Molecular Weight, Plasminogen chemistry, Protein Binding, Streptokinase chemistry, Structure-Activity Relationship, Tissue Plasminogen Activator chemistry, alpha-2-Antiplasmin chemistry, Fibrinolysin chemistry, Streptokinase metabolism

Abstract

Streptokinase (SK) interacts with human plasminogen (Pg) or plasmin (Pm) with formation of Pg-SK or Pm-SK complex. Pm-SK complex manifests a fibrinolytic, amidolytic and Pg activator activity. SK in complex with Pm isn't stable and so capable to be hydrolysed rapidly. We investigated a correlation between molecular form of SK and catalytic properties of equimolar Pm-SK complex during preincubation at 20 degrees C. It was found out that amidolytic activity of Pm-SK complex was not changing for 5 hours and decreased to the initial Pm value after 24 hours. During this time alpha 2-antiplasmin (alpha 2-AP) has any effect on amidolytic activity of the complex. Fibrinolytic activity of Pm-SK complex makes up 20% of the initial Pm value and wasn't changing within the investigated period. Pg activator activity was decreasing rapidly to 30-40% of the initial one within few minutes from the moment of Pm-SK complex formation. It was 10-20% of that initial after 24 hours. The decrease in Pg activator activity of Pm-SK complex correlated with the initial very rapid conversion of 47 kDa SK to 36 kDa SK within few minutes and following more slow conversion of SK in 31, 25 and 15 kDa fragments after 5 hours. alpha 2-AP didn't influence on the Pg activator activity of Pm-SK complex but eliminated its fibrinolytic activity completely. It was supposed that alpha 2-AP inhibited fibrinolytic activity of Pm-SK complex similarly to 6-aminohexanoic acid by preventing Pm-SK complex binding to fibrin polymer.

Published

2002

5. [Features of plasminogen activation in a complex with antiplasminogen monoclonal antibody IV-1C].

Author

Slominsk'kyĭ OIu, Makohonenko IeM, Kolesnikova IM, and Cederholm-Williams SA

Subjects

Amides metabolism, Antibodies, Monoclonal chemistry, Catalysis, Epitopes immunology, Plasminogen chemistry, Plasminogen immunology, Antibodies, Monoclonal immunology, Plasminogen metabolism

Abstract

Antiplasminogen monoclonal antibody IV-1c (IV-1c) with antigenic determinant in V709-G718 site of plasminogen (Pg) protease domain (Druzhina N.N. et al. 1996.) can induce catalytic activity in Pg moiety of the complex. Catalytic activity appeared in Pg-IV-1c complex after approximately 2 h lag-period. Rate of Lys-Pg activation was higher then that of Glu-Pg. Amidolytic activity of Pg-SK equimolar complex was completely inhibited by IV-1c at 2:1 = Pg:IV-1c molar ratio. At constant Glu-Pg concentration increasing of the IV-1c concentration to equimolar of Pg accelerated Pg activation. Subsequent increase of IV-1c concentration inhibited the Pg activation sharply. Increasing of Glu-Pg concentration at constant IV-1c one did not inhibit Glu-Pg activation in Pg-IV-1c complex. The rate dependence of Pg activation from Glu-Pg-IV-1c complex concentration curve had bell-shaped form with maximum at 500 nM. Electrophoretic analysis of components of Glu-Pg-IV-1c complex showed that Lys-Pg and Lys-Pm were not observed at 100 nM complex concentration for 6 h period of reaction. At 680 nM concentration Glu-Pg-IV-1c complex these forms appeared in initial moments of reaction activation after lag-period. Kinetic scheme and peculiarities of Pg activation reaction in Pg-IV-1c complex are discussed.

Published

1999

6. [Plasminogen binding with decapeptide and polypeptide fragments of streptokinase].

Author

Korol'chuk VI, Makohonenko IeM, and Sederkhol'm-Vil'iams SA

Subjects

Amino Acid Sequence, Animals, Cattle, Humans, Immunoenzyme Techniques, Molecular Sequence Data, Peptide Fragments chemistry, Plasminogen chemistry, Protein Binding, Streptokinase chemistry, Swine, Peptide Fragments metabolism, Plasminogen metabolism, Streptokinase metabolism

Abstract

The plasminogen binding with streptokinase decapeptides, modeling the primary structure of molecule, and chymotryptic fragments of streptokinase have been investigated. The immunoenzymatic assay has shown that plasminogen binds to all streptokinase fragments with the decreasing affinity in the set of fragments: 36 > 30 > 17 > 7 > 11 kDa. Location of the binding sites in streptokinase primary structure was performed using the immobilized decapeptides on plastic pins adopted to IEA. In the presence of 10 mM 6-aminohexanoic acid 11 sites for human Glu- and mini-plasminogens, pig and bovine plasminogens binding have been found. They were of the same location for human, bovine and pig plasminogens. 3 sites were located in plasminogen alpha-domain--T43-A72, N113-T126, Q133-V158, 5 sites in beta-domain--T163-L188, A203-S222, Q239-I264, Y275-L294, T315-L340, and 3 sites in gamma-domain--T361-R362, N377-E392, T397-N410. Participation of linear part of streptokinase polypeptide chain in plasminogen--streptokinase complex formation is suggested.

Published

1999

7. [Val709-Glu724 streptokinase binding site on plasminogen interacts with streptokinase sequence Thr361-Arg372 during plasminogen-streptokinase complex formation].

Author

Korol'chuk VI

Subjects

Binding Sites, Humans, Plasminogen chemistry, Plasminogen metabolism, Streptokinase metabolism

Abstract

Localization of the human plasminogen binding site on the streptokinase of complementary Val709-Glu724 plasminogen being crucial one in providing for the plasminogen streptokinase complex activity has been investigated. Experiments were performed with streptokinase fragments and synthetic decapeptides, antiplasminogen monoclonal anti-body IV-1c and synthetic peptide corresponding to Val709-Gly718 sequence of human plasminogen. It was found that plasminogen sequence Val709-Glu724 interacted with Thr361-Arg372 sequence of strepto-kinase.

Published

1999