Human prothrombin activation

Downing, Michael R.; Butkowski, Ralph J.; Clark, Morgan; Mann, Kenneth G.

doi:10.1016/s0021-9258(19)40670-4

Cited by 120 publications

(27 citation statements)

References 40 publications

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“…Proteins. Prothrombin was purified from titrated bovine plasma and from human Cohn fraction 3 (a gift of Dr. Charles Heldebrant, Abbott Laboratories) or from Red Cross factor IX concentrate (gift of Dr. Yu-Lee Hao, the American National Red Cross) as previously described (Downing et al, 1975;. Prothrombin fragment 1 and prethrombin 1 were prepared by proteolytic cleavage of prothrombin by thrombin and were separated as described elsewhere (Downing et al, 1975;Heldebrant et al, 1973).…”

Section: Methodsmentioning

confidence: 99%

“…Prothrombin was purified from titrated bovine plasma and from human Cohn fraction 3 (a gift of Dr. Charles Heldebrant, Abbott Laboratories) or from Red Cross factor IX concentrate (gift of Dr. Yu-Lee Hao, the American National Red Cross) as previously described (Downing et al, 1975;. Prothrombin fragment 1 and prethrombin 1 were prepared by proteolytic cleavage of prothrombin by thrombin and were separated as described elsewhere (Downing et al, 1975;Heldebrant et al, 1973). Prothrombin fragment 2, bovine prethrombin 2, and human prethrombin 2des(1_l3) were prepared by proteolytic cleavage of prethrombin 1 by factor Xa and were separated as previously described (Downing et al, 1975;Heldebrant et al, 1973).…”

Section: Methodsmentioning

confidence: 99%

“…The most readily isolated activation components of bovine and human prothrombin are1 (Mann, 1976) prothrombin 0006-2960/79/0418-1957S01.00/0 © 1979 American Chemical Society fragment 1 and prethrombin 1, produced by the thrombin catalyzed cleavage of prothrombin, and prothrombin fragment 2 and prethrombin 2, produced by a factor Xa catalyzed cleavage of prethrombin 1. The human protein differs from the bovine in that human prothrombin contains an additional thrombin-sensitive site (Downing et al, 1975). This additional site results in the liberation of an amino-terminal peptide of 13 residues from the A chain of human thrombin (and/or prethrombin 2).…”

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confidence: 99%

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Prothrombin domains: circular dichroic evidence for a lack of cooperativity

Bloom¹,

Mann²

1979

Biochemistry

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The far-ultraviolet circular dichroism spectra of bovine and human prothrombin, prothrombin fragment 1, prethrombin 1, prothrombin fragment 2, and prethrombin 2 (prethrombin 2des(1--13)) were determined and the method of Chen et al. [Chen, Y. H., Yang, J. T., & Martinez, H. M. (1972) Biochemistry 11, 4120--4131; Chen, Y. H., Yang, J. T., & Chau, K. H. (1974) Biochemistry 13, 3350--3359] was used to calculate the apparent alpha-helix, beta-sheet, and random-coil contents of each protein. Prothrombin and its activation components were found to contain a large amount of aperiodic secondary structure and there was little species difference between the spectra and, thus, secondary structures. The hypothesis that the prothrombin activation components exist as relative ly noncooperative "domains" within the prothrombin molecule was tested by comparing the circular dichroism spectrum of prothrombin with the sum of the spectra of the components. It support of the hypothesis, no gross alterations in the spectra and, hence, secondary structures of the components were found to have occurred upon activation.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

mentioning

confidence: 99%

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Prothrombin domains: circular dichroic evidence for a lack of cooperativity

Bloom¹,

Mann²

1979

Biochemistry

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“…(B) Electrophoresis of 10 pg of reduced rabbit transferrin under a variety of denaturing conditions; (1) sodium dodecyl sulfate gel electrophoresis, 5% acrylamide; (2) acid-urea system, 10% acrylamide; (3) sodium dodecyl sulfate-urea gel electrophoresis, 12.5% acrylamide. Munkres (1971) as described by Downing et al (1975). Gels were stained for protein using Coomassie brilliant blue, and for carbohydrate by the use of the periodate-Schiff stain (Segrest & Jackson, 1972).…”

Section: Methodsmentioning

confidence: 99%

Structural studies on rabbit transferrin: isolation and characterization of the glycopeptides

Strickland¹,

Hudson²

1978

Biochemistry

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The structure of rabbit transferrin was investigated with regard to number, size, and composition of the heteropolysaccharide units and their relative location on the polypeptide chain. The composition and molecular weight of the Pronase glycopeptides revealed that rabbit transferrin contains two heteropolysaccharide units, each composed of 2 sialic acid residues, 2 galactose residues, 3 mannose residues, and 4-N-acetylglucosamine residues. The composition and molecular weight of the tryptic glycopeptides further substantiated the existence of two identical heteropolysaccharide units and revealed that both units have identical amino acid residues in the immediate vicinity of the carbohydrate attachment sites to the polypeptide chain, suggesting a sequence homology surrounding the two glycosylation sites. Characterization of the cyanogen bromide fragments from rabbit transferrin indicated that both heteropolysaccharide units are located within a single polypeptide fragment representing approximately one-third of the molecule.

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“…139 "Ολοι είναι γλυκοπρωτεΐνες μέ μιά αλυσο καί μοριακό βάρος 72-54.00. 44 ' Ηπατοκυτταρική βλάβη καί χορήγηση κουμαρινικών παραγώγων έχουν σάν αποτέλεσμα τή μειωμένη σύνθεση καί των 4 αυτών παραγόν των, 40 ενώ κατά τή διάρκεια εγκυμοσύνης τά επίπεδα τους αυξάνονται. "Ολοι προσροφώνται άπό τό φωσφορικό ασβέστιο, τό υδροξείδιο τοϋ άργιλίου ή τό θειικό βάριο, όλοι έχουν τήν ίδια σταθερά θερμοκρασίας καί είναι σταθεροί στους -20°C γιά μεγάλο διάστημα, σέ αντίθεση μέ τους πα ράγοντες V καί VIII, πού είναι ασταθείς παράγοντες.…”

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Διαταραχες Της Πηξεως Στην Οξεια Ιογενη Ηπατιτιδα Των Παιδιων

Ζερβη¹

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10 3. Ποσοτικός προσδιορισμός του παράγοντα VII 42 4. Ποσοτικός προσδιορισμός τοΰ παράγοντα II 5. Ποσοτικός προσδιορισμός τοΰ παράγοντα Χ 6. Ποσοτικός προσδιορισμός τοΰ παράγοντα VIII 7. Προσδιορισμός τών προϊόντων άποδόμησης τοΰ Ινώδους 8. Προσδιορισμός τής άντιγονικής δραστηριότητας τοΰ παράγοντα VIII μέ τήν άνοσοτεχνική Laurell 9. Ποσοτικός προσδιορισμός ΑΤΙΠ μέ άνοσοδιάχυση ΑΠΟΤΕΛΕΣΜΑΤΑ ΣΥΖΗΤΗΣΗ ΣΥΜΠΕΡΑΣΜΑΤΑ ΠΕΡΙΛΗΨΗ SUMMARY ΒΙΒΛΙΟΓΡΑΦΙΑ

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Human prothrombin activation

Cited by 120 publications

References 40 publications

Prothrombin domains: circular dichroic evidence for a lack of cooperativity

Prothrombin domains: circular dichroic evidence for a lack of cooperativity

Structural studies on rabbit transferrin: isolation and characterization of the glycopeptides

Διαταραχες Της Πηξεως Στην Οξεια Ιογενη Ηπατιτιδα Των Παιδιων

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